In vitro nephrotoxicity screening assay

ABSTRACT

The invention relates to methods for predicting the in vivo nephrotoxicity of a nucleic acid molecule, in particular a nucleic acid molecule such as a siRNA or an antisense oligonucleotide using an in vitro cell based assay measuring the levels of EGFR as toxicity biomarker, potentially in combination with other biomarkers like ATP and KIM-1.

CROSS REFERENCE TO RELATED APPLICATIONS

This application is a National Phase application under 35 U.S.C. § 371 of PCT International Application number PCT/EP2017/064730 filed Jun. 16, 2017, which claims priority to EP Patent Application No. 16174994.0 filed Jun. 17, 2016. The entire contents of the foregoing applications are hereby incorporated by reference.

FIELD OF INVENTION

The invention relates to methods for predicting the in vivo nephrotoxicity of a nucleic acid molecule, in particular a nucleic acid molecule such as a siRNA, an antisense oligonucleotide or aptamer using an in vitro cell based assay measuring the levels of epidermal growth factor receptor (EGFR) as toxicity biomarker, potentially in combination with other biomarkers like kidney injury molecule-1 (KIM-1) and adenosine triphosphate (ATP). The invention further relates to methods for selecting one or more nucleic acid molecules for in vivo administration from a library of nucleic acid molecules, in particular a nucleic acid molecule such as a RNAi agent, an antisense oligonucleotide or aptamer, using said assay.

BACKGROUND

One of the issues in identification of new as well as optimized drug candidates is the event of dose limiting toxicity. When evaluated in vivo, typically a sub-set of nucleic acid molecule compounds will elicit a toxicity phenotype, such as drug induced kidney injury or nephrotoxicity.

In the past few years a number of models for predicting nephrotoxicity of nucleic acid molecules have been developed using various biomarkers.

Sohn et al 2013 Toxicology letters Vol 217 pp 235 and Huang et al 2015 Pharmacological Research & Perspectives Vol 3 pp e00148 both disclose in vitro cell based assays for the prediction of nephrotoxicity of small molecules using various biomarkers including kidney injury molecule-1 (KIM-1).

Ju et al 2015 Science translational medicine Vol 7, pp 316ra193 describes epidermal growth factor (EGF) as a potential in vivo biomarker for chronic kidney disease by measuring EGF transcript and secretion in the urine correlated to the glomerular filtration rate. There is no description of measuring in vitro EGFR reduction or extracellular EGF uptake.

Wilmer et al 2016 Trends in Biotechnology Vol 34 pp 156 reviews further biomarkers for screening of drug-induced nephrotoxicity both in vivo and in vitro (see table 2).

In vitro nephrotoxicity assays have shown some ability to predict known nephrotoxicity of some small molecule or polypeptide drug substances such as amphotericin B (antifungal agent), colistin (polypeptide antibiotic), ciclosporin (immonosupressant agent), cisplatin (chemotherapeutic agent), doxorubicin (chemotherapeutic agent), gentamicin (anti-bacterial agent).

This has however not been the case for a different class of drugs namely nucleic acid based drugs such as iRNAs, antisense oligonucleotides and aptamers. Nephrotoxicity of individual nucleic acid compounds has been published previously and appears to be unpredictable (see for example Henry et al 1997 Toxicology Vol 120 pp 145; Monteith et al 1999 Toxicologic pathology Vol 27, pp. 307; Herrington et al 2011 American journal of kidney diseases: the official journal of the National Kidney Foundation Vol 57, pp 300; Voit et al. 2014 The Lancet. Neurology Vol 13, pp 987; van Poelgeest et al 2015 British journal of clinical pharmacology Vol 80, pp 1350).

To our knowledge an in vitro cell based assay using EGFR as a biomarker for the prediction of nephrotoxicity of a nucleic acid molecule has not been described. In particular the in vitro prediction of nephrotoxicity of antisense oligonucleotides has not previously been described.

OBJECTIVE OF THE INVENTION

The present invention establishes EGFR as a reliable biomarker in an in vitro cell based assay for prediction of in vivo nephrotoxicity of a nucleic acid molecule, such as an antisense oligonucleotide.

Reliable in vitro predictions of nephrotoxicity would increase the successful clinical development of drugs, and without the use of animals for the initial screening drug discovery will be more cost-effective, efficient and ethical, reducing the number of animals needed for toxicity screening of libraries of nucleic acid molecules significantly.

SUMMARY OF THE INVENTION

The invention provides in vitro toxicity assays which have been found to be predictive for in vivo nephrotoxicity of nucleic acid molecules, in particular oligonucleotides, such as antisense oligonucleotides.

In one aspect of the invention, the present inventors have identified epidermal growth factor receptor (EGFR) as a biomarker of nephrotoxicity. This biomarker can be combined with other biomarkers such as kidney injury molecule-1 (KIM-1).

The invention provides for an in vitro method (an assay) for predicting in vivo toxicity (or in vivo toxicity potential) which may be used to select nucleic acid molecule compounds which are, or are predicted to be, suitable for in vivo administration without adverse nephrotoxicity, such as acute kidney injury or drug-induced kidney injury.

The invention provides for a method for predicting the in vivo nephrotoxicity of a nucleic acid molecule, in particular a nucleic acid based molecule such as an antisense oligonucleotide in a mammal, said method comprising the steps of:

a) culturing cells expressing epidermal growth factor receptor (EGFR) in a suitable cell culture media;

b) administering the nucleic acid molecule to said cell culture;

c) incubating the cells for a period of time; and

d) subsequently measuring the EGFR mRNA level in the cells;

wherein a decrease in EGFR mRNA is indicative of a nucleic acid molecule which is, or is predicted to be, associated with nephrotoxicity

The invention provides for a method for selecting one or more nucleic acid molecules suitable for in vivo administration, from a library of nucleic acid molecules, said method comprising the steps of

-   -   a. obtaining a library of nucleic acid molecules;     -   b. administering each member of the library of nucleic acid         molecules to cell culture expressing epidermal growth factor         receptor (EGFR);     -   c. culturing the cells in vitro for a period of time;     -   d. measuring the amount of intracellular EGFR mRNA for each         nucleic acid molecule; and     -   e. selecting one or more nucleic acid molecules wherein the         reduction in EGFR relative to a control sample is above 80%.

Optionally, the method may further comprise the step of administering the selected nucleic acid molecule in vivo to a mammal.

Suitably, in the methods of the invention the level or amount of the at least one biomarker may be compared to the level obtained when administering a control sample such as vehicle sample or a non-toxic reference nucleic acid molecule (confirmed as non-toxic in vivo) to determine the level of increase or decrease of the at least one biomarker due to the administration of the nucleic acid molecule (i.e. an alteration of the at least one biomarker of nephrotoxicity). Furthermore, the at least one biomarker may be compared to the level obtained when administering a toxic reference nucleic acid molecule (confirmed as toxic in vivo) to determine the assay window of the at least one biomarker.

In some embodiments the cells expressing EGFR is selected from cell cultures originating from epithelial cells, mesenchymal cells and neuroectodermal cells. In particular cell cultures originating from kidney epithelial cells are useful in the methods of the inventions, such as human PTEC or human PTEC-TERT-1 cell cultures.

In some embodiments, the predicted nephrotoxicity is associated with a decrease of EGFR biomarker in the cells. In further embodiments an increase in KIM-1 levels are indicative of a nucleic acid molecule which is, or is predicted to be, associated with nephrotoxicity. Further biomarkers for predicting nephrotoxicity may be associated with a decrease in intracellular ATP levels.

The invention provides for the use of an in vitro assay to determine the (e.g. likely) nephrotoxicity of a nucleic acid molecule, in particular a nucleic acid based molecule, such as an oligonucleotide, such as a LNA oligonucleotide. The invention provides for a nucleic acid molecule obtained by the method for predicting nephrotoxicity of the present invention or by the method for screening a library of nucleic acid molecules.

A pharmaceutical composition comprising the nucleic acid molecule obtained by the method for predicting nephrotoxicity of the present invention or by the method for screening a library of nucleic acid molecules and a pharmaceutically acceptable diluent, solvent, carrier, salt and/or adjuvant.

The nucleic acid molecule obtained by the method for predicting nephrotoxicity of the present invention or by the method for screening a library of nucleic acid molecules or the pharmaceutical composition comprising such a molecule for use in a medicine.

BRIEF DESCRIPTION OF THE FIGURES

FIG. 1 shows morphological changes of PTEC-TERT1 cells treated with 100 μM oligonucleotide for 7 days.

FIG. 2 Schematically illustrates how the EGFR and KIM-1 biomarkers correlate with the toxicity observed in vivo. White indicates no toxicity (innocuous); light gray indicate mild toxicity; intermediate gray indicate medium toxicity; and dark gray indicate high toxicity.

DEFINITIONS Immortalized Cell Line

The term “immortalized cell line” in the context of the present invention is to be understood as a population of cells descended from a single cell in a multicellular organism, where the cells have been modified to escape normal cellular senescence to allow continuous proliferation or division of the cells. Immortalized cells can be grown for prolonged periods in vitro. The mutations required for immortality can occur naturally or be intentionally induced e.g. using viral vectors, deletion of genes, induction of genes or proteins such as telomerases or fusion with immortal cells such as cancer cells.

Primary Cell Culture

The term “primary cell culture” in the context of the present invention is to be understood as a population of cells isolated from a specific tissue in an animal. The primary cell culture is cultivated without prior genetic manipulations or clonal selection, it may however be purified using e.g. FACS or selective growth conditions. The primary cell culture can either be fresh or established from cryopreserved tissue.

Target Nucleic Acid

According to the present invention, the target nucleic acid can be a nucleic acid which encodes a mammalian protein and may for example be a gene, a RNA, a mRNA, and pre-mRNA, a mature mRNA or a cDNA sequence. The target nucleic acid can also be a microRNA, a long-non-coding RNA, a small nucleolar RNA or a transfer RNA.

Nucleic Acid Molecule

The term “nucleic acid molecule” or “therapeutic nucleic acid molecule” as used herein is defined as it is generally understood by the skilled person as a molecule comprising two or more covalently linked nucleosides. The nucleic acid molecule(s) referred to in the method of the invention are generally therapeutic oligonucleotides below 50 nucleotides in length. The nucleic acid molecules may be or comprise an antisense oligonucleotide, or may be another oligomeric nucleic acid molecule, such as a RNAi agent, an aptamer, or a ribozyme. Nucleic acid molecules are commonly made in the laboratory by solid-phase chemical synthesis followed by purification. When referring to a sequence of the nucleic acid molecule, reference is made to the sequence or order of nucleobase moieties, or modifications thereof, of the covalently linked nucleotides or nucleosides. The nucleic acid molecule of the invention is man-made, and is chemically synthesized, and is typically purified or isolated. The nucleic acid molecule of the invention may comprise one or more modified nucleosides or nucleotides.

In some embodiments, the nucleic acid molecule of the invention comprises or consists of 8 to 40 nucleotides in length, such as from 9 to 35, such as from 10 to 30, such as from 11 to 22, such as from 12 to 20, such as from 13 to 18 or 14 to 16 contiguous nucleotides in length.

In some embodiments, the nucleic acid molecule or contiguous nucleotide sequence thereof comprises or consists of 22 or less nucleotides, such as 20 or less nucleotides, such as 18 or less nucleotides, such as 14, 15, 16 or 17 nucleotides. It is to be understood that any range given herein includes the range endpoints. Accordingly, if a nucleic acid molecule is said to include from 10 to 30 nucleotides, both 10 and 30 nucleotides are included.

In some embodiments, the contiguous nucleotide sequence comprises or consists of 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29 or 30 contiguous nucleotides in length

The nucleic acid molecule(s) are typically for modulating the expression of one or more target nucleic acids in a mammal. In some embodiments the nucleic acid molecules, such as for siRNAs and antisense oligonucleotides, are typically for inhibiting the expression of an RNA in a mammal, such as a mRNA or microRNA, for example. The nucleic acid molecules may therefore be effective at modulating the expression of one or more target nucleic acids in a mammal.

In one embodiment of the invention the nucleic acid molecule is selected from a RNAi agents, an antisense oligonucleotide or an aptamer.

In some embodiment the nucleic acid molecule is an antisense oligonucleotide.

In some embodiments the nucleic acid molecule is a phosphorothioate nucleic acid molecule.

In some embodiments the nucleic acid molecule comprises phosphorothioate internucleoside linkages.

In some embodiments the nucleic acid molecule(s) may be conjugated to non-nucleosidic moieties (conjugate moieties).

In some embodiments the nucleic acid molecules used or identified in the method of the invention comprise at least one stereodefined phosphorothioate internucleoside linkage.

A library of nucleic acid molecules is to be understood as a collection of variant nucleic acid molecules. The purpose of the library of nucleic acid molecules can vary. In some embodiments, the library of nucleic acid molecules is composed of oligonucleotides with different nucleobase sequences, for example it may be a library of nucleic acid molecules which are designed across a target nucleic acid (e.g. a RNA sequence), for example a library of antisense oligonucleotides or RNAi agents generated by a mRNA gene-walk with the purpose of identifying regions on the target nucleic acid where nucleic acid molecules efficiently modulate the target nucleic acid. In some embodiments, the library of nucleic acid molecules is composed of oligonucleotides with overlapping nucleobase sequence targeting a specific region on the target nucleic acid with the purpose of identifying the most potent sequence within the library of nucleic acid molecules. In some embodiments, the library of nucleic acid molecules is a library of nucleic acid molecule design variants (child nucleic acid molecules) of a parent or ancestral nucleic acid molecule, wherein the nucleic acid molecule design variants retaining the core nucleobase sequence of the parent nucleic acid molecule. In some embodiments the library of nucleic acid molecule variants (child nucleic acid molecules) differs from the parent nucleic acid molecule in one or more design parameters. The purpose of such a library is to improve the parent nucleic acid molecule, for example in the context of the present application the parent nucleic acid molecule has been found to elicit nephrotoxicity in vivo.

Antisense Oligonucleotides

The term “Antisense oligonucleotide” as used herein is defined as nucleic acid molecules capable of modulating expression of a target gene by hybridizing to a target nucleic acid, in particular to a contiguous sequence on a target nucleic acid. Antisense oligonucleotides generally contain one or more stretches of DNA or DNA-like nucleosides. The antisense oligonucleotides are not essentially double stranded and are therefore not siRNAs. Preferably, the antisense oligonucleotides of the present invention are single stranded.

In some embodiments, the antisense oligonucleotide(s) are capable of recruiting RNaseH, and may, for example be a gapmer oligonucleotide as defined herein, comprising one or more 2′ sugar modified nucleosides in the flanks, such as 2′-O-alkyl-RNA, 2′-O-methyl-RNA, 2′-alkoxy-RNA, 2′-O-methoxyethyl-RNA, 2′-amino-DNA, 2′-fluoro-DNA, arabino nucleic acid (ANA), 2′-fluoro-ANA and LNA nucleosides or mixtures of these (mixed wing gapmer), or may be a gap-breaker oligonucleotide.

In some embodiments, the antisense oligonucleotides are mixmers. Mixmer oligonucleotides typically comprise alternating regions of high affinity 2′ sugar modified nucleosides, such as 2′-O-alkyl-RNA, 2′-O-methyl-RNA, 2′-alkoxy-RNA, 2′-O-methoxyethyl-RNA, 2′-amino-DNA, 2′-fluoro-DNA, arabino nucleic acid (ANA), 2′-fluoro-ANA and LNA nucleosides, with short regions of 1-4 or 1-3 DNA nucleosides. Typically a mixmer will comprise alternating regions with short stretches of DNA, for example [LNA]₁₋₅[DNA]₁₋₃[LNA]₁₋₄[DNA]₁₋₃[LNA]₁₋₄[DNA]₁₋₃.

Various mixmer designs are highly effective, for example when targeting microRNA (antimiRs), microRNA binding sites on mRNAs (Blockmirs) or as splice switching oligomers (ASOs). See for example WO2007/112754 (LNA-AntimiRs™), WO2008/131807 (LNA splice switching oligos).

In some embodiments, the oligonucleotide may be a TINY LNA oligonucleotide of 7-10 nucleotides in length. Such TINY LNAs are disclosed in WO2009/043353, herein incorporated by reference. They are typically use to inhibit microRNAs and microRNA families, and may be full LNA modified (i.e. each nucleoside is a LNA nucleoside). It is also preferred that as with gapmer and mixmer oligonucleotides, the internucleoside linkages comprise phosphorothioate internucleoside linkages, and as with the oligonucleotides referred to herein may be fully phosphorothiolates oligonucleotides.

Antisense oligonucleotides are typically between 7-30 nucleotides in length, such as between 7-10 nucleotides (e.g. TINY LNAs) or 10-14 nucleotides (e.g. shortmers or short gapmers) or 12-20 or 10-22 or 10-24 nucleotides in length.

iRNA

As used herein, the terms “RNAi”, “RNAi agent,” “iRNA agent”, “RNA interference agent” or “siRNA” as used interchangeably herein, refer to a oligonucleotide molecule that contains RNA nucleosides and which mediates the targeted cleavage of a target nucleic acid, such as an RNA transcript, via an RNA-induced silencing complex (RISC) pathway. iRNA directs the sequence-specific degradation of mRNA through a process known as RNA interference (RNAi). The iRNA modulates, e.g., inhibits, the expression of the target nucleic acid in a cell, e.g., a cell within a subject, such as a mammalian subject.

The RNAi agent subjected to the method of the invention can either be a double stranded RNA (dsRNA) or a single stranded RNA molecule that interacts with a target nucleic acid sequence, such as a target RNA sequence, via the RISC pathway to direct the cleavage of the target nucleic acid. Double stranded RNAi agents are generally between 20 and 50 nucleotides in length, such as between 25 and 35 nucleotides in length, and interacts with the endonuclease known as Dicer which is believed to processes dsRNA into 19-23 base pair short interfering RNAs with characteristic two base 3′ overhangs which are then incorporated into an RNA-induced silencing complex (RISC). Double stranded RNAi agents may siRNA molecules composed of a sense stand and and antisense strand forming a duplex together. Alternatively it can be an oligonucleotide that forms a secondary hairpin structure which essentially makes it double stranded in the region of the hairpin, such molecules are also termed shRNA's.

Effective extended forms of Dicer substrates have been described in U.S. Pat. Nos. 8,349,809 and 8,513,207, hereby incorporated by reference. Upon binding to the appropriate target mRNA, one or more endonucleases within the RISC cleave the target to induce silencing. Single-stranded RNAi agents bind to the RISC endonuclease Argonaute 2, which then cleaves the target mRNA. Single-stranded iRNAs are generally 15-30 nucleotides long and are chemically modified, e.g. including modified internucleoside linkages and potentially also modified nucleosides. The design and testing of single-stranded siRNAs are described in U.S. Pat. No. 8,101,348 and in Lima et al., (2012) Cell I 50: 883-894, hereby incorporated by reference. dsRNA's may be chemically modified in the same manner as the single stranded RNAi agents.

Aptamer

As used herein, the term aptamer refers to an oligonucleotide or peptide that forms a three-dimensional structure capable of modulating a target through a ligand-target interaction, such as a ligand-protein interaction or a ligand-DNA helix interaction. Oligonucleotide aptamers can be formed of DNA, RNA or modified nucleosides or a mixture of these. Aptamers are effective via their three dimensional structure not through target hybridization as for antisense oligonucleotides or RNAi agents.

Modified Internucleoside Linkages

Modified internucleoside linkages may, for example, be selected from the group comprising phosphorothioate, diphosphorothioate and boranophosphate. In some embodiments, the modified internucleoside linkages are compatible with the RNaseH recruitment of the oligonucleotide to be tested in the method of the invention, for example phosphorothioate, diphosphorothioate or boranophosphate.

In some embodiments the internucleoside linkage comprises sulphur (S), such as a phosphorothioate internucleoside linkage. In some embodiments the oligonucleotides used or identified in the method of the invention comprise at least one stereodefined phosphorothioate internucleoside linkage.

A phosphorothioate internucleoside linkage is particularly useful due to nuclease resistance, beneficial pharmakokinetics and ease of manufacture. In some embodiments at least 50% of the internucleoside linkages in the oligonucleotide, or contiguous nucleotide sequence thereof, are phosphorothioate, such as at least 60%, such as at least 70%, such as at least 80 or such as at least 90% of the internucleoside linkages in the oligonucleotide, or contiguous nucleotide sequence thereof, are phosphorothioate. In some embodiments all of the internucleoside linkages of the oligonucleotide, or contiguous nucleotide sequence thereof, are phosphorothioate.

In some embodiments, the oligonucleotide comprises one or more neutral internucleoside linkage, particularly an internucleoside linkage selected from phosphotriester, methylphosphonate, MMI, amide-3, formacetal or thioformacetal.

Further internucleoside linkages are disclosed in WO2009/124238 (incorporated herein by reference). In an embodiment the internucleoside linkage is selected from linkers disclosed in WO2007/031091 (incorporated herein by reference). Particularly, the internucleoside linkage may be selected from —O—P(O)₂—O—, —O—P(O,S)—O—, —O—P(S)₂—O—, —S—P(O)₂—O—, —S—P(O,S)—O—, —S—P(S)₂—O—, —O—P(O)₂—S—, —O—P(O,S)—S—, —S—P(O)₂—S—, —O—PO(RH)—O—, 0-PO(OCH₃)-0-, —O—PO(NRH)—O—, —O—PO(OCH₂CH₂S—R)—O—, —O—PO(BH₃)—O—, —O—PO(NHRH)—O—, —O—P(O)₂—NRH—, —NRH—P(O)₂—O—, —NRH—CO—O—, —NRH—CO—NRH—, and/or the internucleoside linker may be selected form the group consisting of: —O—CO—O—, —O—CO—NRH—, —NRH—CO—CH₂—, —O—CH₂—CO—NRH—, —O—CH₂—CH₂—NRH—, —CO—NRH—CH₂—, —CH₂—NRHCO—, —O—CH₂—CH₂—S—, —S—CH₂—CH₂—O—, —S—CH₂—CH₂—S—, —CH₂—SO₂—CH₂—, —CH₂—CO—NRH—, —O—CH₂—CH₂—NRH—CO—, —CH₂—NCH₃—O—CH₂—, where RH is selected from hydrogen and C₁₋₄-alkyl.

Nuclease resistant linkages, such as phosphothioate linkages, are particularly useful in oligonucleotide regions capable of recruiting nuclease when forming a duplex with the target nucleic acid, such as region G for gapmers, or the non-modified nucleoside region of headmers and tailmers. Phosphorothioate linkages may, however, also be useful in non-nuclease recruiting regions and/or affinity enhancing regions such as regions F and F′ for gapmers, or the modified nucleoside region of headmers and tailmers.

Each of the design regions may however comprise internucleoside linkages other than phosphorothioate, such as phosphodiester linkages, in particularly in regions where modified nucleosides, such as LNA, protect the linkage against nuclease degradation. Inclusion of phosphodiester linkages, such as one or two linkages, particularly between or adjacent to modified nucleoside units (typically in the non-nuclease recruiting regions) can modify the bioavailability and/or bio-distribution of an oligonucleotide—see WO2008/113832, incorporated herein by reference.

In an embodiment all the internucleoside linkages in the oligonucleotide are phosphorothioate and/or boranophosphate linkages. In some embodiment, all the internucleoside linkages in the oligonucleotide are phosphorothioate linkages.

Stereodefined Internucleotide Linkages

In the context of the present invention the term “stereodfined” refers to nucleic acid molecules, such as oligonucleotides including antisense, RNI and aptamer molecules, where at least one phosphorothioate internucleoside linkage present in the oligonucleotide has defined stereochemistry, i.e. either Rp or Sp. In some embodiments all of the phosphorothioate internucleoside linkages in a stereodefined oligonucleotide may be stereodefined, i.e. each phosphorothioate internucleoside linkage is independently selected from the group consisting of Rp and Sp phosphorothioate internucleoside linkages.

Typically, oligonucleotide phosphorothioates are synthesised as a random mixture of Rp and Sp phosphorothioate linkages (also referred to as a racemic mixture). In the present invention, gapmer phosphorothioate oligonucleotides are provided where at least one of the phosphorothioate linkages of the gap region oligonucleotide is stereodefined, i.e. is either Rp or Sp in at least 75%, such as at least 80%, or at least 85%, or at least 90% or at least 95%, or at least 97%, such as at least 98%, such as at least 99%, or (essentially) all of the oligonucleotide molecules present in the oligonucleotide sample. Such oligonucleotides may be referred as being stereodefined, stereoselective or stereospecified: They comprise at least one phosphorothioate linkage which is stereospecific. The terms stereodefined and stereospecified/stereoselective may be used interchangeably herein. The terms stereodefined, stereoselective and stereospecified may be used to describe a phosphorothioate internucleoside linkage (Rp or Sp), or may be used to described a oligonucleotide which comprises such a phosphorothioate internucleoside linkage. It is recognized that a stereodefined oligonucleotide may comprise a small amount of the alternative stereoisomer at any one position, for example Wan et al reports a 98% stereoselectivity for the gapmers reported in NAR, November 2014.

Modulation of Expression

The term “modulation of expression” as used herein is to be understood as an overall term for an oligonucleotide's ability to alter the amount of a nucleic acid target when compared to the amount of the nucleic acid target before administration of the oligonucleotide. Alternatively modulation of expression may be determined by reference to a control experiment. It is generally understood that the control is an individual or target cell treated with a saline composition or an individual or target cell treated with a non-targeting oligonucleotide (mock). It may however also be an individual treated with the standard of care.

One type of modulation is an oligonucleotide's ability to inhibit, down-regulate, reduce, suppress, remove, stop, block, prevent, lessen, lower, avoid or terminate expression of the nucleic acid target e.g. by degradation of mRNA or blockage of transcription. Another type of modulation is an oligonucleotide's ability to restore, increase or enhance expression of nucleic acid target e.g. by repair of splice sites or prevention of splicing or removal or blockage of inhibitory mechanisms such as microRNA repression.

In some embodiments of the invention, when the target of the oligonucleotide of the invention is present in the EGFR expressing cells, the method of the invention may further comprise the step of determining the level of target modulation (e.g. inhibit for siRNAs or antisense oligonucleotides) in the population of EGFR expressing cells after treatment with the oligonucleotides (e.g. this may occur in parallel or as part of the measurement of the at least one biomarker step). In this regard the method of the invention may be used to determine the comparative potency or effectiveness of the oligonucleotide and the comparative toxicity, allowing for the selection of potent non-toxic compounds for use in vivo. It will be understood that the determination of compound potency/effectiveness may be performed in a separate in vitro experiment, either in the EGFR expressing cells, particularly cells which are expressing the target.

Modified Oligonucleotides

Non modified DNA and RNA molecules are rapidly degraded in vivo, and as such are of little use therapeutically. Typically, the oligonucleotide(s) used in the method of the invention are therefore modified. One widely used modification is the use of phosphorothioate internucleoside linkages, which is known to stabilise oligonucleotides from nucleolytic degradation, as well as providing desirable pharmacological properties. In some embodiments the oligonucleotide(s) comprise phosphorothioate internucleoside linkages.

Another desirable modification are those which confer higher affinity of the oligonucleotide to the target nucleic acid, so called high affinity modified nucleotides, which include bicyclic “LNA” nucleosides as well as numerous 2′ substituted nucleosides.

High Affinity Modified Nucleosides

In some embodiments, the oligonucleotide comprises one or more high affinity modified nucleoside. A high affinity modified nucleoside is a modified nucleoside which, when incorporated into the oligonucleotide enhances the affinity of the oligonucleotide for its complementary target, for example as measured by the melting temperature (T^(m)). A high affinity modified nucleoside of the present invention preferably result in an increase in melting temperature between +0.5 to +12° C., more preferably between +1.5 to +10° C. and most preferably between +3 to +8° C. per modified nucleoside. Numerous high affinity modified nucleosides are known in the art and include for example 2′ sugar modified nucleosides, such as many 2′ substituted nucleosides as well as locked nucleic acids (LNA) (see e.g. Freier & Altmann; Nucl. Acid Res., 1997, 25, 4429-4443 and Uhlmann; Curr. Opinion in Drug Development, 2000, 3(2), 293-213).

Sugar Modifications

The oligonucleotide(s) may comprise one or more nucleosides which have a modified sugar moiety, i.e. a modification of the sugar moiety when compared to the ribose sugar moiety found in naturally occurring DNA and RNA nucleosides.

Numerous nucleosides with modification of the ribose sugar moiety have been made, primarily with the aim of improving certain properties of oligonucleotides, such as affinity and/or nuclease resistance. Such modifications include those where the ribose ring structure is modified, e.g. by replacement with a hexose ring (HNA).

Sugar modifications also include modifications made via altering the substituent groups on the ribose ring to groups other than hydrogen, or the 2′-OH group naturally found in DNA and RNA nucleosides. Substituents may, for example be introduced at the 2′, 3′, 4′ or 5′ positions of the ribose ring. Nucleosides with modified sugar moieties also include 2′ modified nucleosides, such as 2′ substituted nucleosides. Numerous 2′ substituted nucleosides have been found to have beneficial properties when incorporated into oligonucleotides, such as enhanced nucleoside resistance and enhanced affinity. In one embodiment the nucleic acid molecule(s) or library of such molecules comprises one or more 2′ sugar modified nucleoside.

In addition to the 2′ substitution there are other modifications including a modification at position 2 of the ribose ring, such as introduction of a bicyclic ring, which typically have a biradicle bridge between the C2 and C4 carbons on the ribose ring (also known as locked nucleic acid or LNA), or an unlinked ribose ring which typically lacks a bond between the C2 and C3 carbons (e.g. UNA). Other sugar modified nucleosides include, for example, bicyclohexose nucleic acids (WO2011/017521) or tricyclic nucleic acids (WO2013/154798). Modified nucleosides also include nucleosides where the sugar moiety is replaced with a non-sugar moiety, for example in the case of peptide nucleic acids (PNA), or morpholino nucleic acids.

2′ Sugar Modified Nucleosides

A 2′ sugar modified nucleoside is a nucleoside which has a substituent other than H or —OH at the 2′ position (2′ substituted nucleoside) or comprises a 2′ linked biradicle, and includes 2′ substituted nucleosides and LNA (2′-4′ biradicle bridged) nucleosides. For example, the 2′ modified sugar may provide enhanced binding affinity and/or increased nuclease resistance to the oligonucleotide. Examples of 2′ substituted modified nucleosides are 2′-O-alkyl-RNA, 2′-O-methyl-RNA, 2′-alkoxy-RNA, 2′-O-methoxyethyl-RNA (MOE), 2′-amino-DNA, 2′-Fluoro-RNA, and 2′-F-ANA nucleoside. For further examples, please see e.g. Freier & Altmann; Nucl. Acid Res., 1997, 25, 4429-4443 and Uhlmann; Curr. Opinion in Drug Development, 2000, 3(2), 293-213, and Deleavey and Damha, Chemistry and Biology 2012, 19, 937. Below are illustrations of some 2′ substituted modified nucleosides.

Locked Nucleic Acid Nucleosides (LNA)

In some embodiments oligonucleotides are LNA oligonucleotides, i.e. they comprise at least one LNA nucleoside.

LNA monomers (also referred to as bicyclic nucleic acids, BNA) are nucleosides where there is a biradical between the 2′ and 4′ position of the ribose ring. The 2′-4′ biradical is also referred to as a bridge. LNA monomers, when incorporated into a oligonucleotides are known to enhance the binding affinity of the oligonucleotide to a complementary DNA or RNA sequence, typically measured or calculated as an increase in the temperature required to melt the oligonucleotide/target duplex (T_(m)).

The LNA oligomer may be a single stranded antisense oligonucleotide.

The LNA used in the oligonucleotide compounds of the invention may have the structure of the general formula I

wherein for all chiral centers, asymmetric groups may be found in either R or S orientation;

wherein X is selected from —O—, —S—, —N(R^(N*))—, —C(R⁶R^(6*))—, such as, in some embodiments —O—;

B is selected from hydrogen, optionally substituted C₁₋₄-alkoxy, optionally substituted C₁₋₄-alkyl, optionally substituted C₁₋₄-acyloxy, nucleobases including naturally occurring and nucleobase analogues, DNA intercalators, photochemically active groups, thermochemically active groups, chelating groups, reporter groups, and ligands; preferably, B is a nucleobase or nucleobase analogue;

P designates an internucleotide linkage to an adjacent monomer, or a 5′-terminal group, such internucleotide linkage or 5′-terminal group optionally including the substituent R⁵ or equally applicable the substituent R^(5*);

P* designates an internucleotide linkage to an adjacent monomer, or a 3′-terminal group;

R^(4*) and R^(2*) together designate a bivalent linker group consisting of 1-4 groups/atoms selected from —C(R^(a)R^(b))—, —C(R^(a))═C(R^(b))—, —C(R^(a))═N—, —O—, —Si(R^(a))₂—, —S—, —SO₂—, —N(R^(a))—, and >C═Z, wherein Z is selected from —O—, —S—, and —N(R^(a))—, and R^(a) and R^(b) each is independently selected from hydrogen, optionally substituted C₁₋₁₂-alkyl, optionally substituted C₂₋₁₂-alkenyl, optionally substituted C₂₋₁₂-alkynyl, hydroxy, optionally substituted C₁₋₁₂-alkoxy, C₂₋₁₂-alkoxyalkyl, C₂₋₁₂-alkenyloxy, carboxy, C₁₋₁₂-alkoxycarbonyl, C₁₋₁₂-alkylcarbonyl, formyl, aryl, aryloxy-carbonyl, aryloxy, arylcarbonyl, heteroaryl, heteroaryloxy-carbonyl, heteroaryloxy, heteroarylcarbonyl, amino, mono- and di(C₁₋₆-alkyl)amino, carbamoyl, mono- and di(C₁₋₆-alkyl)-amino-carbonyl, amino-C₁₋₆-alkyl-aminocarbonyl, mono- and di(C₁₋₆-alkyl)amino-C₁₋₆-alkyl-aminocarbonyl, C₁₋₆-alkyl-carbonylamino, carbamido, C₁₋₆-alkanoyloxy, sulphono, C₁₋₆-alkylsulphonyloxy, nitro, azido, sulphanyl, C₁₋₆-alkylthio, halogen, DNA intercalators, photochemically active groups, thermochemically active groups, chelating groups, reporter groups, and ligands, where aryl and heteroaryl may be optionally substituted and where two geminal substituents R^(a) and R^(b) together may designate optionally substituted methylene (═CH₂), wherein for all chiral centers, asymmetric groups may be found in either R or S orientation, and;

each of the substituents R^(1*), R², R³, R⁵, R^(5*), R⁶ and R^(6*), which are present is independently selected from hydrogen, optionally substituted C₁₋₁₂-alkyl, optionally substituted C₂₋₁₂-alkenyl, optionally substituted C₂₋₁₂-alkynyl, hydroxy, C₁₋₁₂-alkoxy, C₂₋₁₂-alkoxyalkyl, C₂₋₁₂-alkenyloxy, carboxy, C₁₋₁₂-alkoxycarbonyl, C₁₋₁₂-alkylcarbonyl, formyl, aryl, aryloxy-carbonyl, aryloxy, arylcarbonyl, heteroaryl, heteroaryloxy-carbonyl, heteroaryloxy, heteroarylcarbonyl, amino, mono- and di(C₁₋₆-alkyl)amino, carbamoyl, mono- and di(C₁₋₆-alkyl)-amino-carbonyl, amino-C₁₋₆-alkyl-aminocarbonyl, mono- and di(C₁₋₆-alkyl)amino-C₁₋₆-alkyl-aminocarbonyl, C₁₋₆-alkyl-carbonylamino, carbamido, C₁₋₆-alkanoyloxy, sulphono, C₁₋₆-alkylsulphonyloxy, nitro, azido, sulphanyl, C₁₋₆-alkylthio, halogen, DNA intercalators, photochemically active groups, thermochemically active groups, chelating groups, reporter groups, and ligands, where aryl and heteroaryl may be optionally substituted, and where two geminal substituents together may designate oxo, thioxo, imino, or optionally substituted methylene; wherein R^(N) is selected from hydrogen and C₁₋₄-alkyl, and where two adjacent (non-geminal) substituents may designate an additional bond resulting in a double bond; and R^(N*), when present and not involved in a biradical, is selected from hydrogen and C₁₋₄-alkyl; and basic salts and acid addition salts thereof. For all chiral centers, asymmetric groups may be found in either R or S orientation.

In some embodiments, R^(4*) and R^(2*) together designate a biradical consisting of a groups selected from the group consisting of C(R^(a)R^(b))—C(R^(a)R^(b))—, C(R^(a)R^(b))—O—, C(R^(a)R^(b))—NR^(a)—, C(R^(a)R^(b))—S—, and C(R^(a)R^(b))—C(R^(a)R^(b))—O—, wherein each R^(a) and R^(b) may optionally be independently selected. In some embodiments, R^(a) and R^(b) may be, optionally independently selected from the group consisting of hydrogen and _(C1-6)alkyl, such as methyl, such as hydrogen.

In some embodiments, R^(4*) and R^(2*) together designate the biradical —O—CH(CH₂OCH₃)-(2′O-methoxyethyl bicyclic nucleic acid—Seth at al., 2010, J. Org. Chem)—in either the R— or S— configuration.

In some embodiments, R^(4*) and R^(2*) together designate the biradical —O—CH(CH₂CH₃)-(2′O-ethyl bicyclic nucleic acid—Seth at al., 2010, J. Org. Chem).—in either the R— or S— configuration.

In some embodiments, R^(4*) and R^(2*) together designate the biradical —O—CH(CH₃)—.—in either the R— or S— configuration. In some embodiments, R^(4*) and R^(2*) together designate the biradical —O—CH₂—O—CH₂— —(Seth at al., 2010, J. Org. Chem).

In some embodiments, R^(4*) and R^(2*) together designate the biradical —O—NR—CH₃— —(Seth at al., 2010, J. Org. Chem).

In some embodiments, the LNA units have a structure selected from the following group:

In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are independently selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl. For all chiral centers, asymmetric groups may be found in either R or S orientation.

In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are hydrogen.

In some embodiments, R^(1*), R², R³ are independently selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl. For all chiral centers, asymmetric groups may be found in either R or S orientation.

In some embodiments, R^(1*), R², R³ are hydrogen.

In some embodiments, R⁵ and R^(5*) are each independently selected from the group consisting of H, —CH₃, —CH₂—CH₃, —CH₂—O—CH₃, and —CH═CH₂. Suitably in some embodiments, either R⁵ or R^(5*) are hydrogen, where as the other group (R⁵ or R^(5*) respectively) is selected from the group consisting of C₁₋₅ alkyl, C₂₋₆ alkenyl, C₂₋₆ alkynyl, substituted C₁₋₆ alkyl, substituted C₂₋₆ alkenyl, substituted C₂₋₆ alkynyl or substituted acyl (—C(═O)—); wherein each substituted group is mono or poly substituted with substituent groups independently selected from halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl, substituted C₂₋₆ alkynyl, OJ₁, SJ₁, NJ₁J₂, N₃, COOJ₁, CN, O—C(═O)NJ₁J₂, N(H)C(═NH)NJ,J₂ or N(H)C(═X)N(H)J₂ wherein X is O or S; and each J₁ and J₂ is, independently, H, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl, substituted C₂₋₆ alkynyl, C₁₋₆ aminoalkyl, substituted C₁₋₆ aminoalkyl or a protecting group. In some embodiments either R⁵ or R^(5*) is substituted C₁₋₆ alkyl. In some embodiments either R⁵ or R^(5*) is substituted methylene wherein preferred substituent groups include one or more groups independently selected from F, NJ₁J₂, N₃, CN, OJ₁, SJ₁, O—C(═O)NJ₁J₂, N(H)C(═NH)NJ, J₂ or N(H)C(O)N(H)J₂. In some embodiments each J₁ and J₂ is, independently H or C₁₋₆ alkyl. In some embodiments either R⁵ or R^(5*) is methyl, ethyl or methoxymethyl. In some embodiments either R⁵ or R^(5*) is methyl. In a further embodiment either R⁵ or R^(5*) is ethylenyl. In some embodiments either R⁵ or R^(5*) is substituted acyl. In some embodiments either R⁵ or R^(5*) is C(═O)NJ₁J₂. For all chiral centers, asymmetric groups may be found in either R or S orientation. Such 5′ modified bicyclic nucleotides are disclosed in WO 2007/134181, which is hereby incorporated by reference in its entirety.

In some embodiments B is a nucleobase, including nucleobase analogues and naturally occurring nucleobases, such as a purine or pyrimidine, or a substituted purine or substituted pyrimidine, such as a nucleobase referred to herein, such as a nucleobase selected from the group consisting of adenine, cytosine, thymine, adenine, uracil, and/or a modified or substituted nucleobase, such as 5-thiazolo-uracil, 2-thio-uracil, 5-propynyl-uracil, 2′thio-thymine, 5-methyl cytosine, 5-thiozolo-cytosine, 5-propynyl-cytosine, and 2,6-diaminopurine.

In some embodiments, R^(4*) and R^(2*) together designate a biradical selected from —C(R^(a)R^(b))—O—, —C(R^(a)R^(b))—C(R^(c)R^(d))—O—, —C(R^(a)R^(b))—C(R^(c)R^(d))—C(R^(e)R^(f))—O—, —C(R^(a)R^(b))—O—C(R^(c)R^(d))—, —C(R^(a)R^(b))—O—C(R^(c)R^(d))—O—, —C(R^(a)R^(b))—C(R^(c)R^(d))—, —C(R^(a)R^(b))—C(R^(c)R^(d))—C(R^(e)R^(f))—, —C(R^(a))═C(R^(b))—C(R^(c)R^(d))—, —C(R^(a)R^(b))—N(R^(c))—, —C(R^(a)R^(b))—C(R^(c)R^(d))—N(R^(e))—, —C(R^(a)R^(b))—N(R^(c))—O—, and —C(R^(a)R^(b))—S—, —C(R^(a)R^(b))—C(R^(c)R^(d))—S—, wherein R^(a), R^(b), R^(c), R^(d), R^(e), and R^(f) each is independently selected from hydrogen, optionally substituted C₁₋₁₂-alkyl, optionally substituted C₂₋₁₂-alkenyl, optionally substituted C₂₋₁₂-alkynyl, hydroxy, C₁₋₁₂-alkoxy, C₂₋₁₂-alkoxyalkyl, C₂₋₁₂-alkenyloxy, carboxy, C₁₋₁₂-alkoxycarbonyl, C₁₋₁₂-alkylcarbonyl, formyl, aryl, aryloxy-carbonyl, aryloxy, arylcarbonyl, heteroaryl, heteroaryloxy-carbonyl, heteroaryloxy, heteroarylcarbonyl, amino, mono- and di(C₁₋₆-alkyl)amino, carbamoyl, mono- and di(C₁₋₆-alkyl)-amino-carbonyl, amino-C₁₋₆-alkyl-aminocarbonyl, mono- and di(C₁₋₆-alkyl)amino-C₁₋₆-alkyl-aminocarbonyl, C₁₋₆-alkyl-carbonylamino, carbamido, C₁₋₆-alkanoyloxy, sulphono, C₁₋₆-alkylsulphonyloxy, nitro, azido, sulphanyl, C₁₋₆-alkylthio, halogen, DNA intercalators, photochemically active groups, thermochemically active groups, chelating groups, reporter groups, and ligands, where aryl and heteroaryl may be optionally substituted and where two geminal substituents R^(a) and R^(b) together may designate optionally substituted methylene (═CH₂). For all chiral centers, asymmetric groups may be found in either R or S orientation.

In a further embodiment R^(4*) and R^(2*) together designate a biradical (bivalent group) selected from —CH₂—O—, —CH₂—S—, —CH₂—NH—, —CH₂—N(CH₃)—, —CH₂—CH₂—O—, —CH₂—CH(CH₃)—, —CH₂—CH₂—S—, —CH₂—CH₂—NH—, —CH₂—CH₂—CH₂—, —CH₂—CH₂—CH₂—O—, —CH₂—CH₂—CH(CH₃)—, —CH═CH—CH₂—, —CH₂—O—CH₂—O—, —CH₂—NH—O—, —CH₂—N(CH₃)—O—, —CH₂—O—CH₂—, —CH(CH₃)—O—, and —CH(CH₂—O—CH₃)—O—, and/or, —CH₂—CH₂—, and —CH═CH— For all chiral centers, asymmetric groups may be found in either R or S orientation.

In some embodiments, R^(4*) and R^(2*) together designate the biradical C(R^(a)R^(b))—N(R^(c))—O—, wherein R^(a) and R^(b) are independently selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl, such as hydrogen, and; wherein R^(c) is selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl, such as hydrogen.

In some embodiments, R^(4*) and R^(2*) together designate the biradical C(R^(a)R^(b))—O—C(R^(c)R^(d))—O—, wherein R^(a), R^(b), R^(c), and R^(d) are independently selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl, such as hydrogen.

In some embodiments, R^(4*) and R^(2*) form the biradical —CH(Z)—O—, wherein Z is selected from the group consisting of C₁₋₆ alkyl, C₂₋₆ alkenyl, C₂₋₆ alkynyl, substituted C₁₋₆ alkyl, substituted C₂₋₆ alkenyl, substituted C₂₋₆ alkynyl, acyl, substituted acyl, substituted amide, thiol or substituted thio; and wherein each of the substituted groups, is, independently, mono or poly substituted with optionally protected substituent groups independently selected from halogen, oxo, hydroxyl, OJ₁, NJ₁J₂, SJ₁, N₃, OC(═X)J₁, OC(═X)NJ₁J₂, NJ³C(═X)NJ₁J₂ and CN, wherein each J₁, J₂ and J₃ is, independently, H or C₁₋₆ alkyl, and X is O, S or NJ₁. In some embodiments Z is C₁₋₆ alkyl or substituted C₁₋₆ alkyl. In some embodiments Z is methyl. In some embodiments Z is substituted C₁₋₆ alkyl. In some embodiments said substituent group is C₁₋₆ alkoxy. In some embodiments Z is CH₃OCH₂—. For all chiral centers, asymmetric groups may be found in either R or S orientation. Such bicyclic nucleotides are disclosed in U.S. Pat. No. 7,399,845 which is hereby incorporated by reference in its entirety. In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are hydrogen. In some some embodiments, R^(1*), R², R^(3*) are hydrogen, and one or both of R⁵, R^(5*) may be other than hydrogen as referred to above and in WO 2007/134181.

In some embodiments, R^(4*) and R^(2*) together designate a biradical which comprise a substituted amino group in the bridge such as consist or comprise of the biradical —CH₂—N(R^(c))—, wherein R^(c) is C₁₋₁₂ alkyloxy. In some embodiments R^(4*) and R^(2*) together designate a biradical —Cq₃q₄-NOR—, wherein q₃ and q₄ are independently selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl; wherein each substituted group is, independently, mono or poly substituted with substituent groups independently selected from halogen, OJ₁, SJ₁, NJ₁J₂, COOJ₁, CN, O—C(═O)NJ₁J₂, N(H)C(═NH)N J₁J₂ or N(H)C(═X═N(H)J₂ wherein X is O or S; and each of J₁ and J₂ is, independently, H, C₁₋₆ alkyl, C₂₋₆ alkenyl, C₂₋₆ alkynyl, C₁₋₆ aminoalkyl or a protecting group. For all chiral centers, asymmetric groups may be found in either R or S orientation. Such bicyclic nucleotides are disclosed in WO2008/150729 which is hereby incorporated by reference in its entirety. In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are independently selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl. In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are hydrogen. In some embodiments, R^(1*), R², R³ are hydrogen and one or both of R⁵, R^(5*) may be other than hydrogen as referred to above and in WO 2007/134181. In some embodiments R^(4*) and R^(2*) together designate a biradical (bivalent group) C(R^(a)R^(b))—O—, wherein R^(a) and R^(b) are each independently halogen, C₁-C₁₂ alkyl, substituted C₁-C₁₂ alkyl, C₂-C₁₂ alkenyl, substituted C₂-C₁₂ alkenyl, C₂-C₁₂ alkynyl, substituted C₂-C₁₂ alkynyl, C₁-C₁₂ alkoxy, substituted C₁-C₁₂ alkoxy, OJ₁ SJ₁, SOJ₁, SO₂J₁, NJ₁J₂, N₃, CN, C(═O)OJ₁, C(═O)NJ₁J₂, C(═O)J₁, O—C(═O)NJ₁J₂, N(H)C(═NH)NJ₁J₂, N(H)C(═O)NJ₁J₂ or N(H)C(═S)NJ₁J₂; or R^(a) and R^(b) together are ═C(q3)(q4); q₃ and q₄ are each, independently, H, halogen, C₁-C₁₂ alkyl or substituted C₁-C₁₂ alkyl; each substituted group is, independently, mono or poly substituted with substituent groups independently selected from halogen, C₁-C₆ alkyl, substituted C₁-C₆ alkyl, C₂-C₆ alkenyl, substituted C₂-C₆ alkenyl, C₂-C₆ alkynyl, substituted C₂-C₆ alkynyl, OJ₁, SJ₁, NJ₁J₂, N₃, CN, C(═O)OJ₁, C(═O)NJ₁J₂, C(═O)J₁, O—C(═O)NJ₁J₂, N(H)C(═O)NJ₁J₂ or N(H)C(═S)NJ₁J_(2.) and; each J₁ and J₂ is, independently, H, C1-C₆ alkyl, substituted C1-C₆ alkyl, C₂-C₆ alkenyl, substituted C₂-C₆ alkenyl, C₂-C₆ alkynyl, substituted C₂-C₆ alkynyl, C1-C₆ aminoalkyl, substituted C1-C₆ aminoalkyl or a protecting group. Such compounds are disclosed in WO2009006478A, hereby incorporated in its entirety by reference.

In some embodiments, R^(4*) and R^(2*) form the biradical -Q-, wherein Q is C(q₁)(q₂)C(q₃)(q₄), C(q₁)═C(q₃), C[═C(q₁)(q₂)]-C(q₃)(4₄) or C(q₁)(q₂)-C[═C(q₃)(q₄)]; q₁, q₂, q₃, q₄ are each independently. H, halogen, C₁₋₁₂ alkyl, substituted C₁₋₁₂ alkyl, C₂₋₁₂ alkenyl, substituted C₁₋₁₂ alkoxy, OJ₁, SJ₁, SOJ₁, SO₂J₁, NJ₁J₂, N₃, CN, C(═O)OJ₁, C(═O)—NJ₁J₂, C(═O) J₁, —C(═O)NJ₁J₂, N(H)C(═NH)NJ₁J₂, N(H)C(═O)NJ₁J₂ or N(H)C(═S)NJ₁J₂; each J₁ and J₂ is, independently, H, C₁₋₆ alkyl, C₂₋₆ alkenyl, C₂₋₆ alkynyl, C₁₋₆ aminoalkyl or a protecting group; and, optionally wherein when Q is C(q₁)(q₂)(q₃)(q₄) and one of q₃ or q₄ is CH₃ then at least one of the other of q₃ or q₄ or one of q₁ and q₂ is other than H. In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are hydrogen. For all chiral centers, asymmetric groups may be found in either R or S orientation. Such bicyclic nucleotides are disclosed in WO2008/154401 which is hereby incorporated by reference in its entirety. In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are independently selected from the group consisting of hydrogen, halogen, C₁₋₆ alkyl, substituted C₁₋₆ alkyl, C₂₋₆ alkenyl, substituted C₂₋₆ alkenyl, C₂₋₆ alkynyl or substituted C₂₋₆ alkynyl, C₁₋₆ alkoxyl, substituted C₁₋₆ alkoxyl, acyl, substituted acyl, C₁₋₆ aminoalkyl or substituted C₁₋₆ aminoalkyl. In some embodiments, R^(1*), R², R³, R⁵, R^(5*) are hydrogen. In some embodiments, R^(1*), R², R³ are hydrogen and one or both of R⁵, R^(5*) may be other than hydrogen as referred to above and in WO 2007/134181 or WO2009/067647 (alpha-L-bicyclic nucleic acids analogs).

Further bicyclic nucleoside analogues and their use in antisense oligonucleotides are disclosed in WO2011 115818, WO2011/085102, WO2011/017521, WO09100320, WO10036698, WO09124295 & WO09006478. Such nucleoside analogues may in some aspects be useful in the compounds of present invention.

In some embodiments the LNA used in the oligonucleotide compounds of the invention preferably has the structure of the general formula II:

wherein Y is selected from the group consisting of —O—, —CH₂O—, —S—, —NH—, N(R^(e)) and/or —CH₂—; Z and Z* are independently selected among an internucleotide linkage, R^(H), a terminal group or a protecting group; B constitutes a natural or non-natural nucleotide base moiety (nucleobase), and R^(H) is selected from hydrogen and C₁₋₄-alkyl; R^(a), R^(b) R^(c), R^(d) and R^(e) are, optionally independently, selected from the group consisting of hydrogen, optionally substituted C₁₋₁₂-alkyl, optionally substituted C₂₋₁₂-alkenyl, optionally substituted C₂₋₁₂-alkynyl, hydroxy, C₁₋₁₂-alkoxy, C₂₋₁₂-alkoxyalkyl, C₂₋₁₂-alkenyloxy, carboxy, C₁₋₁₂-alkoxycarbonyl, C₁₋₁₂-alkylcarbonyl, formyl, aryl, aryloxy-carbonyl, aryloxy, arylcarbonyl, heteroaryl, heteroaryloxy-carbonyl, heteroaryloxy, heteroarylcarbonyl, amino, mono- and di(C₁₋₆-alkyl)amino, carbamoyl, mono- and di(C₁₋₆-alkyl)-amino-carbonyl, amino-C₁₋₆-alkyl-aminocarbonyl, mono- and di(C₁₋₆-alkyl)amino-C₁₋₆-alkyl-aminocarbonyl, C₁₋₆-alkyl-carbonylamino, carbamido, C₁₋₆-alkanoyloxy, sulphono, C₁₋₆-alkylsulphonyloxy, nitro, azido, sulphanyl, C₁₋₆-alkylthio, halogen, DNA intercalators, photochemically active groups, thermochemically active groups, chelating groups, reporter groups, and ligands, where aryl and heteroaryl may be optionally substituted and where two geminal substituents R^(a) and R^(b) together may designate optionally substituted methylene (═CH₂); and R^(H) is selected from hydrogen and C₁₋₄-alkyl. In some embodiments R^(a), R^(b) R^(c), R^(d) and R^(e) are, optionally independently, selected from the group consisting of hydrogen and C₁₋₆ alkyl, such as methyl. For all chiral centers, asymmetric groups may be found in either R or S orientation, for example, two exemplary stereochemical isomers include the beta-D and alpha-L isoforms, which may be illustrated as follows:

Specific exemplary LNA units are shown below:

The term “thio-LNA” comprises a locked nucleotide in which Y in the general formula above is selected from S or —CH₂—S—. Thio-LNA can be in both beta-D and alpha-L-configuration.

The term “amino-LNA” comprises a locked nucleotide in which Y in the general formula above is selected from —N(H)—, N(R)—, CH₂—N(H)—, and —CH₂—N(R)— where R is selected from hydrogen and C₁₋₄-alkyl. Amino-LNA can be in both beta-D and alpha-L-configuration.

The term “oxy-LNA” comprises a locked nucleotide in which Y in the general formula above represents —O—. Oxy-LNA can be in both beta-D and alpha-L-configuration.

The term “ENA” comprises a locked nucleotide in which Y in the general formula above is —CH₂—O— (where the oxygen atom of —CH₂—O— is attached to the 2′-position relative to the base B). R^(e) is hydrogen or methyl.

In some exemplary embodiments LNA is selected from beta-D-oxy-LNA, alpha-L-oxy-LNA, beta-D-amino-LNA and beta-D-thio-LNA, in particular beta-D-oxy-LNA.

Certain examples of LNA nucleosides are presented in Scheme 1.

As illustrated in the examples, in some embodiments of the invention the LNA nucleosides in the oligonucleotides are beta-D-oxy-LNA nucleosides.

Gapmer

The term “gapmer” as used herein refers to an antisense oligonucleotide which comprises a region of RNase H recruiting oligonucleotides (gap) which is flanked 5′ and 3′ by regions which comprise one or more affinity enhancing modified nucleosides (flanks or wings). Various gapmer designs are described herein. Headmers and tailmers are oligonucleotides capable of recruiting RNase H where one of the flanks is missing, i.e. only one of the ends of the oligonucleotide comprises affinity enhancing modified nucleosides. For headmers the 3′ flank is missing (i.e. the 5′ flank comprises affinity enhancing modified nucleosides) and for tailmers the 5′ flank is missing (i.e. the 3′ flank comprises affinity enhancing modified nucleosides).

Gapmer Designs

Gapmer oligonucleotides are widely used to inhibit a target RNA in a cell, such as a mRNA or viral RNA, via an antisense mechanism (and may therefore also be called antisense gapmer oligonucleotides). In a gapmer structure the oligonucleotide comprises at least three distinct structural regions a 5′-flank, a gap and a 3′-flank, F-G-F′ in ‘5->3’ orientation. The G region or gap region comprises a region of at least 5 contiguous nucleotides which are capable or recruiting RNaseH, such as a region of DNA nucleotides, e.g. 6-14 DNA nucleotides or other nucleosides which are capable of recruiting RNase H, e.g., alpha-L-oxy-LNA, 2′-Flouro-ANA and UNA. The gap region is flanked 5′ and 3′ by regions (F and F′ also termed flanking regions or wing regions) which comprise one or more affinity enhancing modified nucleosides, such as 2′ modified nucleotides. In some embodiments, the flanking regions may be 1-8 nucleotides in length.

In further embodiments region F (5′ flank or 5′ wing) is attached to the ‘5 end of region G and region F’ (3′ flank or 3′ wing) is attached to the ‘3 end of region G. Region F and F’, comprises contains or consists independently of at least one modified nucleoside such as at least 2, at least 3, at least 4, at least 5, at least 6, at least 7 modified nucleosides. In an embodiment region F and/or F′ comprises or consists independently of from 1 to 7 modified nucleosides, such as from 2 to 6 modified nucleosides, such as from 2 to 5 modified nucleosides, such as from 2 to 4 modified nucleosides, such as from 1 to 3 modified nucleosides, such as 1, 2, 3 or 4 modified nucleosides. The F region is defined by having at least on modified nucleoside at the 5′ end and at the 3′ end of the region. The F′ region is defined by having at least on modified nucleoside at the 5′ end and at the 3′ end of the region.

In some embodiments, the modified nucleosides in region F and/or F′ have a 3′ endo structure.

In an embodiment, one or more of the modified nucleosides in region F and/or F′ are 2′ modified nucleosides. In one embodiment all the nucleosides in Region F and/or F′ are 2′ modified nucleosides.

In another embodiment region F and/or F′ comprises DNA and/or RNA in addition to the 2′ modified nucleosides. Flanks comprising DNA and/or RNA are characterized by having a 2′ modified nucleoside in the 5′ end and the 3′ end of the F and/or F′ region. In one embodiment the region F and/or F′ comprises DNA nucleosides, such as from 1 to 3 contiguous DNA nucleosides, such as 1 to 3 or 1 to 2 contiguous DNA nucleosides. The DNA nucleosides in the flanks should preferably not be able to recruit RNase H. In some embodiments the 2′ modified nucleosides and DNA and/or RNA nucleosides in the F and/or F′ region alternate with 1 to 3 2′ modified nucleosides and 1 to 3 DNA and/or RNA nucleosides. Such flanks can also be termed alternating flanks. The length of region F and/or F′ in oligonucleotides with alternating flanks may independently be 4 to 10 nucleosides, such as 4 to 8, such as 4 to 6 nucleosides, such as 4, 5, 6 or 7 modified nucleosides. In some embodiments only the F region of the oligonucleotide is alternating. In some embodiments only the F′ region of the oligonucleotide is alternating.

Specific examples of region F and/or F′ with alternating nucleosides are 2′₁₋₃-N′₁₋₄-2′₁₋₃ 2′₁₋₂-N′₁₋₂-2′₁₋₂-N′₁₋₂-2′₁₋₂

Where 2′ indicates a modified nucleoside and N′ is a RNA or DNA. In some embodiments all the modified nucleosides in the alternating flanks are LNA and the N′ is DNA. In a further embodiment one or more of the 2′ modified nucleosides in region F and/or F′ are independently selected from 2′-O-alkyl-RNA units, 2′-O-methyl-RNA, 2′-amino-DNA units, 2′-fluoro-DNA units, 2′-alkoxy-RNA, MOE units, LNA units, arabino nucleic acid (ANA) units and 2′-fluoro-ANA units.

In some embodiments the F and/or F′ region comprises both LNA and a 2′ substituted modified nucleoside. These are often termed mixed wing or mixed flank oligonucleotides.

In one embodiment of the invention all the modified nucleosides in region F and/or F′ are LNA nucleosides. In a further embodiment all the nucleosides in Region F and/or F′ are LNA nucleosides. In a further embodiment the LNA nucleosides in region F and/or F′ are independently selected from the group consisting of oxy-LNA, thio-LNA, amino-LNA, cET, and/or ENA, in either the beta-D or alpha-L configurations or combinations thereof. In a preferred embodiment region F and/or F′ comprise at least 1 beta-D-oxy LNA unit, at the 5′ end of the contiguous sequence.

In further embodiments, Region G (gap region) preferably comprise, contain or consist of at least 4, such as at least 5, such as at least 6, at least 7, at least 8, at least 9, at least 10, at least 11, at least 12, at least 13, at least 14, at least 15 or at least 16 consecutive nucleosides capable of recruiting the aforementioned nuclease, in particular RNaseH. In a further embodiment region G comprise, contain or consist of from 5 to 12, or from 6 to 10 or from 7 to 9, such as 8 consecutive nucleotide units capable of recruiting aforementioned nuclease.

The nucleoside units in region G, which are capable of recruiting nuclease are in an embodiment selected from the group consisting of DNA, alpha-L-LNA, C4′ alkylated DNA (as described in PCT/EP2009/050349 and Vester et al., Bioorg. Med. Chem. Lett. 18 (2008) 2296-2300, both incorporated herein by reference), arabinose derived nucleosides like ANA and 2′F-ANA (Mangos et al. 2003 J. AM. CHEM. SOC. 125, 654-661), UNA (unlocked nucleic acid) (as described in Fluiter et al., Mol. Biosyst., 2009, 10, 1039 incorporated herein by reference). UNA is unlocked nucleic acid, typically where the bond between C2 and C3 of the ribose has been removed, forming an unlocked “sugar” residue.

In a still further embodiment at least one nucleoside unit in region G is a DNA nucleoside unit, such as from 1 to 12 DNA units, such as 2, 3, 4, 5, 6, 7, 8, 9, 10 or 11 DNA units, preferably from 2 to 12 DNA units, such as from 4 to 12 DNA units, more preferably from 5 to 11, or from 2 to 10, 4 to 10 or 6 to 10 DNA units, such as from 7 to 10 DNA units, most preferably 8, 9 or 10 DNA units. In some embodiments, region G consists of 100% DNA units.

In further embodiments the region G may consist of a mixture of DNA and other nucleosides capable of mediating RNase H cleavage. Region G may consist of at least 50% DNA, more preferably 60%, 70% or 80% DNA, and even more preferred 90% or 95% DNA.

In a still further embodiment at least one nucleoside unit in region G is an alpha-L-LNA nucleoside unit, such as at least one alpha-L-LNA, such as 2, 3, 4, 5, 6, 7, 8 or 9 alpha-L-LNA. In a further embodiment, region G comprises the least one alpha-L-LNA is alpha-L-oxy-LNA. In a further embodiment region G comprises a combination of DNA and alpha-L-LNA nucleoside units.

In some embodiments the size of the contiguous sequence in region G may be longer, such as 12, 13, 14, 15, 16, 17, 18, 19 or 20 nucleoside units.

In some embodiments, nucleosides in region G have a 2′ endo structure.

In the gapmer designs reported herein the gap region (Y′) may comprise one or more stereodefined phosphorothaiote linkage, and the remaining internucleoside linkages of the gap region may e.g. be non-stereodefined internucleoside linkages, or may also be stereodefined phosphorothioate linkages.

LNA Gapmer

The term LNA gapmer is a gapmer oligonucleotide wherein at least one of the affinity enhancing modified nucleosides is an LNA nucleoside. In some embodiments both flanks of the gapmer oligonucleotide comprise at least one LNA unit, and in some embodiments, all of the nucleoside of the flanks are LNA nucleosides.

In some embodiments, the 3′ flank comprises at least one LNA nucleoside, preferably at least 2 LNA nucleosides. In some embodiments, the 5′ flank comprises at least one LNA nucleoside. In some embodiments both the 5′ and 3′ flanking regions comprise a LNA nucleoside. In some embodiments all the nucleosides in the flanking regions are LNA nucleosides. Typically the LNA load of the flanks of LNA gapmers is lower than that for 2′ substituted nucleosides, and examples of LNA gapmer designs include [LNA]₁₋₄-[DNA]₅₋₁₅-[LNA]₁₋₄. In some embodiments, the gapmer is a so-called shortmer as described in WO2008/113832 incorporated herein by reference.

Further gapmer designs are disclosed in WO2004/046160, WO2007/146511 and incorporated by reference.

Mixed Wing Gapmer

The term mixed wing gapmer or mixed flank gapmer refers to a LNA gapmer wherein at least one of the flank regions comprise at least one LNA nucleoside and at least one non-LNA modified nucleoside, such as at least one DNA nucleoside or at least one 2′ substituted modified nucleoside, such as, for example, 2′-O-alkyl-RNA, 2′-O-methyl-RNA, 2′-alkoxy-RNA, 2′-O-methoxyethyl-RNA (MOE), 2′-amino-DNA, 2′-Fluoro-RNA and 2′-F-ANA nucleoside(s). In some embodiments the mixed wing gapmer has one flank which comprises only LNA nucleosides (e.g. 5′ or 3′) and the other flank (3′ or 5′ respectfully) comprises 2′ substituted modified nucleoside(s) and optionally LNA nucleosides.

Gapbreaker

The term “gapbreaker oligonucleotide” is used in relation to a gapmer capable of maintaining RNAseH recruitment even though the gap region is disrupted by a non-RNaseH recruiting nucleoside (a gap-breaker nucleoside, E) such that the gap region comprise less than 5 consecutive DNA nucleosides. Non-RNaseH recruiting nucleosides are for example nucleosides in the 3′ endo conformation, such as LNA's where the bridge between C2′ and C4′ of the ribose sugar ring of a nucleoside is in the beta conformation, such as beta-D-oxy LNA or ScET nucleoside. The ability of gapbreaker oligonucleotide to recruit RNaseH is typically sequence or even compound specific—see Rukov et al. 2015 Nucl. Acids Res. Vol. 43 pp. 8476-8487, which discloses “gapbreaker” oligonucleotides which recruit RNaseH which in some instances provide a more specific cleavage of the target RNA.

In some embodiments, the oligonucleotide of the invention is a gapbreaker oligonucleotide. In some embodiments the gapbreaker oligonucleotide comprise a 5′-flank (F), a gap (G) and a 3′-flank (F′), wherein the gap is disrupted by a non-RNaseH recruiting nucleoside (a gap-breaker nucleoside, E) such that the gap contain at least 3 or 4 consecutive DNA nucleosides. The gap-breaker design is based upon the gapmer designs, e.g. those disclosed here (e.g. Region F corresponds to the X′ region of the gapmer above, and region F′ corresponds to the region Z′ of the gapmer described herein), with the exception that the gap region (region Y′) comprises a gap-breaker nucleoside. In some embodiments the gapbreaker nucleoside (E) is an LNA nucleoside where the bridge between C2′ and C4′ of the ribose sugar ring of a nucleoside is in the beta conformation and is placed within the gap region such that the gap-breaker LNA nucleoside is flanked 5′ and 3′ by at least 3 (5′) and 3 (3′) or at least 3 (5′) and 4 (3′) or at least 4(5′) and 3(3′) DNA nucleosides, and wherein the oligonucleotide is capable of recruiting RNaseH.

The gapbreaker oligonucleotide can be represented by the following formulae: F-G-E-G-F′; in particular F₁₋₇-G₃₋₄-E₁-G₃₋₄-F′₁₋₇ D′-F-G-F′, in particular D′₁₋₃-F₁₋₇-G₃₋₄-E₁-G₃₋₄-F′₁₋₇ F-G-F′-D″, in particular F₁₋₇-G₃₋₄-E₁-G₃₋₄-F′₁₋₇-D″₁₋₃ D′-F-G-F′-D″, in particular D′₁₋₃-F₁₋₇-G₃₋₄-E₁-G₃₋₄-F′₁₋₇-D″₁₋₃

Where G represents DNA nucleosides and region D′ and D″ are optional and may additional 5′ and/or 3′ nucleosides, such as DNA nucleosides.

In some embodiments the gapbreaker nucleoside (E) is a LNA, beta-D-oxy LNA or ScET or another LNA nucleoside, such as beta-D-nucleoside disclosed herein.

Stereodefined Gapmers

In some embodiments, the child oligonucleotides originating from a parent gapmer oligonucleotide has at least one of the internucleoside linkages of the gap region which is stereodefined, and optionally wherein the gap region comprises both Rp and Sp internucleoside linkages.

In some embodiments, in the child oligonucleotide(s) (and optionally the parent), at least one of the internucleoside linkages of the gap region are stereodefined, and wherein the central region comprises both Rp and Sp internucleoside linkages.

In some embodiments, in the child oligonucleotide(s) (and optionally the parent), the internucleoside linkages within region G are all stereodefined phosphorothioate internucleoside linkages. In some embodiments, in the child oligonucleotide(s) (and optionally the parent), the internucleoside linkages within region F and F′ are stereodefined phosphorothioate internucleoside linkages. In some embodiments in the child oligonucleotide(s) (and optionally the parent), the internucleoside linkages between region F and G and between region G and F′ are stereodefined phosphorothioate internucleoside linkages. In some embodiments in the child oligonucleotide(s) (and optionally the parent), all the internucleoside linkages within the contiguous nucleosides of regions F-G-F′ are stereodefined phosphorothioate internucleoside linkages.

The introduction of at least one stereodefined phosphorothioate linkages in the gap region of an oligonucleotide may be used to modulate the biological profile of the oligonucleotide, for example it may modulate the toxicity profile. In some embodiments, 2, 3, 4 or 5 of the phosphorothioate linkages in the gap region in the child oligonucleotide(s) (and optionally the parent), are stereodefined. In some embodiments the remaining internucleoside linkages in the gap region are not stereodefined: They exist as a racemic mixture of Rp and Sp in the population of oligonucleotide species. In some embodiments in the child oligonucleotide(s) (and optionally the parent), the remaining internucleoside linkage in the oligonucleotide are not stereodefined. In some embodiments in the child oligonucleotide(s) (and optionally the parent), all the internucleoside linkages in the gap region are stereodefined.

In some embodiments 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, or 14 of the linkages in the gap region of the oligomer are stereoselective phosphorothioate linkages.

In some embodiments 5%, 10%, 15%, 20%, 25%, 30%, 35%, 40%, 45%, 50%, 55%, 60%, 65%, 70%, 75%, 80%, 85%, 90%, or 95% of the linkages in the oligomer (e.g. gapmer) are stereoselective phosphorothioate linkages. In some embodiments all of the phosphorothioate linkages in the oligomer are stereoselective phosphorothioate linkages. In some embodiments the all the internucleoside linkages of the oligomer are stereodefined phosphorothioate linkages.

RNase H Activity and Recruitment

The RNase H activity of an antisense oligonucleotide refers to its ability to recruit RNase H when in a duplex with a complementary RNA molecule. WO01/23613 provides in vitro methods for determining RNaseH activity, which may be used to determine the ability to recruit RNaseH. Typically an oligonucleotide is deemed capable of recruiting RNase H if it, when provided with a complementary target nucleic acid sequence, has an initial rate, as measured in pmol/l/min, of at least 5%, such as at least 10% or more than 20% of the of the initial rate determined when using a oligonucleotide having the same base sequence as the modified oligonucleotide being tested, but containing only DNA monomers with phosphorothioate linkages between all monomers in the oligonucleotide, and using the methodology provided by Example 91-95 of WO01/23613 (hereby incorporated by reference).

Efficacy and Therapeutic Index

The nucleic acid molecules identified by the method of the invention may in addition the toxicity be tested as part of the method of the invention to determine that they are still effective nucleic acid molecules. In particular with nucleic acid based nucleic acid molecules it has been observed that when toxicity is reduced this is in part due to a reduction in the efficacy of the nucleic acid molecule. In one aspect of the invention the decrease in the toxicity grade does not result in a significant decrease in the efficacy. In some embodiments the therapeutic index (TI) of the nucleic acid molecule selected according to the method of the invention is improved when compared to a toxic reference substance. For the purpose of the present invention TI refers to the dose of the nucleic acid molecule that causes adverse effects in the kidney in 50% of subjects (TD50) divided by the dose that leads to the desired efficacy (target knockdown or pharmacological effect) in 50% of subjects (EC50). In some embodiments the TI is increased by at least 10%, such as at least 15, 25, 50, 75, 100, 150, 200, 250 or 300% when compared to a toxic reference nucleic acid molecule, such as Compound 4-1 herein or a toxic parent oligonucleotide or toxic parent nucleic acid molecule. For experimental purposes, assuming the target is present in mice, TD50 and EC50 may be determined in mice in a seven day mouse study. If for example for nucleic acid molecules, the sequence conservation in mice is unfavorable, other model species may be used, e.g. rat, monkey, dog, pig or monkey (e.g. cynomolgus monkey). In some embodiments the increase in TI is due to an increased TD50 and a low or no decrease in EC50. The increase in TI may also be the result of improvements on both parameters. In relation to the method of the invention the increase in TI is not brought about by only improving the efficacy of the nucleic acid molecule (i.e. reduced EC50).

The method of the invention may therefore comprise an additional step of screening the library of (e.g. child) nucleic acid molecules for their efficacy in modulating, e.g. inhibiting, their target. Alternatively, the method of the invention may comprise an additional step of testing the selected nucleic acid molecules (e.g. stereodefined oligonucleotide variants) with a reduced toxicity to determine their efficacy as nucleic acid molecules, e.g. as antisense oligonucleotides. For antisense oligonucleotides the efficacy may be determined by the oligonucleotides ability to recruit RNaseH, or in some embodiments may be the ability to modulate the expression of the target in a cell, in vitro, or in some embodiments, in vivo.

Conjugate Moieties

In some embodiments, the conjugate moiety comprises or is a carbohydrate, non nucleosidic sugars, carbohydrate complexes. In some embodiments, the carbohydrate is selected from the group consisting of galactose, lactose, n-acetylgalactosamine, mannose, and mannose-6-phosphate.

In some embodiments, the conjugate moiety comprises or is selected from the group of protein, glycoproteins, polypeptides, peptides, antibodies, enzymes, and antibody fragments,

In some embodiments, the conjugate moiety is a lipophilic moiety such as a moiety selected from the group consisting of lipids, phospholipids, fatty acids, and sterols.

In some embodiments, the conjugate moiety is selected from the group consisting of small molecules drugs, toxins, reporter molecules, and receptor ligands.

In some embodiments, the conjugate moiety is a polymer, such as polyethyleneglycol (PEG), polypropylene glycol.

In some embodiments the conjugate moiety is or comprises a asialoglycoprotein receptor targeting moiety, which may include, for example galactose, galactosamine, N-formyl-galactosamine, Nacetylgalactosamine, N-propionyl-galactosamine, N-n-butanoyl-galactosamine, and N-isobutanoylgalactos-amine. In some embodiments the conjugate moiety comprises a galactose cluster, such as N-acetylgalactosamine trimer. In some embodiments, the conjugate moiety comprises a GalNAc (N-acetylgalactosamine), such as a mono-valent, di-valent, tri-valent of tetra-valent GalNAc. Trivalent GalNAc conjugates may be used to target the compound to the liver (see e.g. U.S. Pat. No. 5,994,517 and Hangeland et al., Bioconjug Chem. 1995 November-December; 6(6):695-701, WO2009/126933, WO2012/089352, WO2012/083046, WO2014/118267, WO2014/179620, & WO2014/179445), see specific examples in FIG. 2. These GalNAc references and the specific conjugates used therein are hereby incorporated by reference.

DETAILED DESCRIPTION OF THE INVENTION Prediction of In Vivo Toxicity

The methods described herein may be used to predict the in vivo toxicity of a nucleic acid molecule in a mammal. Toxicity of any compound is typically dependent upon its dose, and as such the methods of the invention may be used to assess a compounds comparative toxicity profile as compared to a negative control, and/or a nucleic acid molecule whose toxicity profile is known, or compared to a population (or a library) of nucleic acid molecules, such as a library of nucleic acid molecules, in particular a library of antisense oligonucleotides. In this respect, the prediction of in vivo toxicity may be an assessment of the comparative risk of encountering a toxicity phenotype, such as nephrotoxicity, when the nucleic acid molecule(s) are administered in vivo in a mammal.

When assessing the safety of a nucleic acid molecule, in particular an antisense oligonucleotide, one of the parameters that is investigated is the impact of the substance on the kidney, e.g. accumulation in renal proximal tubules, tubular degenerative/regenerative changes (tubulotoxicity), biomarkers for acute kidney injury, like KIM-1, which are detectable in the urine. Kidney related toxicities are generally known as nephrotoxicity.

The methods of the invention may be used to predict the in vivo toxicity (e.g. nephrotoxicity), or alternatively stated to determine the likely in vivo toxicity profile (e.g. nephrotoxicity), of a nucleic acid molecule in vivo in a mammal. In one embodiment of the invention the in vivo nephrotoxicity is acute kidney injury and/or tubular degradation. The methods of the invention may be used to identify nucleic acid molecules which are not toxic (e.g. not nephrotoxic) in vivo, when used at dosages which are effective in modulating their target, or at therapeutically effective doses. The methods of the present invention therefore allows the selection of nucleic acid molecules which do not exhibit dose limiting toxicity (e.g. nephrotoxicity) when used in vivo at effective dosages. It will be recognized that it is an advantage to have a wide safety margin when selecting nucleic acid molecules for in vivo or for therapeutic use, and as such the methods of the invention may be used to identify or select nucleic acid molecules which do not elicit in vivo toxicity, such as nephrotoxicity, when dosed effectively, or at higher doses, e.g. at up to 2× the effective dose, or up to 3× the effective dose, or up to 5× the effective dose, or up to 10× the effective dose. The methods of the invention may therefore be used to identify nucleic acid molecules for in vivo use which have a maximum tolerated dose higher (e.g. at least 2×, at least 3×, at least 5×, at least 10×) than the effective dose. In this regard the methods of the invention may be used to select nucleic acid molecules which have a suitable therapeutic index (TI) for safe therapeutic administration, or an improved therapeutic index as defined herein.

The present invention establishes EGFR as a reliable biomarker in an in vitro cell based assay for prediction of in vivo nephrotoxicity of a nucleic acid molecule.

One aspect of the present invention is an in vitro method for predicting in vivo nephrotoxicity of a nucleic acid molecule in a mammal, said method comprising the steps of:

-   -   a) culturing cells expressing epidermal growth factor receptor         (EGFR) in a suitable cell culture media;     -   b) administering the nucleic acid molecule to said cell culture;     -   c) incubating the cells for a period of time; and     -   d) subsequently measuring the EGFR mRNA level in the cells;

wherein a decrease in EGFR mRNA in the cells is indicative of a nucleic acid molecule which is, or is predicted to be, associated with nephrotoxicity.

The decrease in intracellular EGFR mRNA levels can be evaluated in relation to a reference value (control) obtained from non-treated cells, cells treated with vehicle (vehicle control, i.e the solvent in which the nucleic acid molecule is dissolved, e.g. saline, DMSO or other suitable solvents) or cells treated with non-toxic reference nucleic acid molecule where the non-toxic nucleic acid molecule has been validated as non-toxic in vivo (an in vivo validated non-toxic nucleic acid molecule). Such a non-toxic nucleic acid molecule can for example be antisense oligonucleotide compound 1-1 with SEQ ID NO: 1, in particular if the nucleic acid molecule(s) that is being subjected to the assay of the invention is a nucleic acid molecule(s), such as an antisense oligonucleotide(s).

In some embodiments, the alteration in the EGFR biomarker is determined as the percentage of the reference value. As is illustrated in the examples, the present inventors have found that a decrease in the level of EGFR mRNA in the cells (intra cellular EGFR) below 80%, such as below 75%, such as below 70%, such as below 60%, such as below 50%, such as below 40% relative to the reference value is predicative of nephrotoxicity of the drug compound. In embodiments where the nucleic acid molecule is an antisense oligonucleotide the oligonucleotide is administered to the cells in a concentration above 10 micro molar, such as between 20 and 150 micro molar, such as between 30 and 120 micro molar, such as between 50 and 100 micro molar.

In further embodiments the EGFR mRNA level in the cells is further compared to a second reference value obtained from cells treated with a nephrotoxic nucleic acid molecule, where the nephrotoxic reference nucleic acid molecule has been validated to cause nephrotoxicity in vivo (an in vivo validated nephrotoxic reference nucleic acid molecule). In some embodiments, the method of the invention may therefore further comprise the method steps of the invention using the administration of one or more nucleic acid molecules with a known toxicity (e.g. nephrotoxicity) profile, such as a positive control nucleic acid molecule which is known to elicit in vivo nephrotoxicity and/or a negative control nucleic acid molecule which is known not to elicit in vivo nephrotoxicity, and a comparison of the level of EGFR mRNA in the cells from the administration of the nucleic acid molecule(s) with the levels obtained from the positive and/or negative controls. The generation of data from of a negative control (vehicle control or in vivo validated non-toxic nucleic acid molecule) and a positive control (in vivo validated nephrotoxic nucleic acid molecule) allows determination of an assay window that can be used to normalize for batch to batch variation in the assay. The assay window (AW) is the difference between the non-toxic reference nucleic acid molecule and the nephrotoxic reference nucleic acid molecule.

In one embodiment the decrease in the level of EGFR mRNA is assed using the conditions for oligonucleotide treatment described in the “materials and methods” section where the oligonucleotide is administered to the cells in a concentration above 1 micro molar, such as above 5 micro molar, such as above 10 micro molar, such as between 20 and 150 micro molar, such as between 30 and 120 micro molar, such as between 50 and 100 micro molar.

In some embodiment the in vivo validated nephrotoxic reference nucleic acid molecule is antisense oligonucleotide compound 4-1 with SEQ ID NO: 4.

In addition or alternatively, the control data may be determined by comparing a library of nucleic acid molecules, in particular a library of nucleic acid molecules such as antisense oligonucleotides, RNAi agents or aptamers, using the method of the invention, either in series or in parallel, and comparing the level of EGFR mRNA biomarker after administration of each member of the library of nucleic acid molecules. Such a method allows for the selection of comparatively less toxic (such as nephrotoxic) nucleic acid molecules. In some embodiments, the control data may be or may include control data which is from a cell culture sample which has not been administered a nucleic acid molecule or vehicle control (day 0 control). Such a sample may be obtained immediately prior to the administration step.

Complementary Biomarkers

As is illustrated in the examples, the present inventors have found that extracellular kidney injury molecule-1 (KIM-1) protein levels or intracellular KIM-1mRNA levels can serve as complementary biomarkers to the EGFR biomarker further strengthening the predictability of the method of the invention.

In some examples the EGFR biomarker alone was not sufficient to predict the nephrotoxicity of a compound with known in vivo nephrotoxicity. In these instances KIM-1 as an in vitro biomarker showed to complement the EGFR biomarker very well. As illustrated in FIG. 2 the combination of EGFR and KIM-1 biomarkers in the assay of the invention resulted in a 100% prediction of compounds with known in vivo nephrotoxicity.

In an embodiment of the invention the method for predicting in vivo nephrotoxicity of a nucleic acid molecule in a mammal, said method comprising the steps of:

-   -   a) culturing cells expressing epidermal growth factor receptor         (EGFR) in a suitable cell culture media;     -   b) administering the nucleic acid molecule to said cell culture;     -   c) incubating the cells for a period of time; and     -   d) subsequently measuring the EGFR mRNA level in the cells and         the KIM-1 protein levels in the supernatant;

wherein a decrease in the EGFR mRNA level or an increase in the KIM-1 level in the supernatant is indicative of a nucleic acid molecule which is, or is predicted to be, associated with nephrotoxicity.

As an alternative or supplement to the extracellular KIM-1 protein levels the intracellular level of KIM-1 mRNA may also be measured.

In some embodiments, the alteration in the KIM-1 protein biomarker is determined as the percentage of the reference value (control) obtained from non-treated cells, cells treated with vehicle (vehicle control, i.e the solvent in which the nucleic acid molecule is dissolved, e.g. saline, DMSO or other suitable solvents) or cells treated with non-toxic reference nucleic acid molecule where the non-toxic nucleic acid molecule has been validated as non-toxic in vivo (an in vivo validated non-toxic nucleic acid molecule). As is illustrated in the examples, the present inventors have found that an increase in the level of KIM-1 in the supernatant (extracellular KIM-1) above 175%, such as at least 200%, such as at least 250%, such as at least 300%, such as at least 350%, such as at least 400% relative to the reference value is predicative of nephrotoxicity of the drug compound. In some embodiments, the alteration in the intracellular KIM-mRNA biomarker is determined as the percentage of the control reference value. As is illustrated in the examples, the present inventors have found that an increase in the level of KIM-1 mRNA in the cells (intracellular KIM-1) above 500%, such as at least 750%, such as at least 1000%, such as at least 1100%, such as at least 1300%, such as at least 1500%, such as at least 1700%, such as at least 2000% relative to the reference value is predicative of nephrotoxicity of the drug compound. An increase in KIM-1 levels is predictive even if there for the same compound is no observable decrease in EGFR levels. Without being bound by theory we suspect that the mechanism that elicits the KIM-1 biomarker increase in vitro is different from the mechanism that elicits the increase in extracellular EGFR levels.

In addition to the EGFR and KIM-1 biomarkers, the inventors have identified an additional biomarkers that can supplement the EGFR biomarker if the cell culture media comprise at least 4 ng/ml of epidermal growth factor (EGF). The additional biomarker is intracellular adenosine triphosphate (ATP).

In a further aspect of the invention ATP can be used as a supplemental biomarker to EGFR in an in vitro cell based assay for prediction of in vivo nephrotoxicity of a nucleic acid molecule.

In another embodiment of the invention the method for predicting in vivo nephrotoxicity of a nucleic acid molecule in a mammal, said method comprising the steps of:

-   -   a) culturing cells expressing epidermal growth factor receptor         (EGFR) in a suitable cell culture media containing at least 4         ng/ml of epidermal growth factor (EGFR);     -   b) administering the nucleic acid molecule to said cell culture;     -   c) incubating the cells for a period of time; and     -   d) subsequently measuring the intracellular EGFR mRNA level and         the intracellular ATP levels;

wherein an decrease in the EGFR mRNA level in the cells and a decrease in the intracellular ATP protein level is indicative of a nucleic acid molecule which is, or is predicted to be, associated with nephrotoxicity.

A decrease of cellular ATP in relation to the control to at least 80%, such at least about 70%, such as at least about 60%, such as at least 50%, such as at least 40% relative to the reference value is indicative of an enhanced propensity to trigger nephrotoxicity in vivo. The ATP biomarker is compared to a set of controls as already described in relation to the EGFR biomarker. In particular to a negative control reference value obtained from non-treated cells, cells treated with vehicle (vehicle control, i.e the solvent in which the nucleic acid molecule is dissolved, e.g. saline, DMSO or other suitable solvents) or cells treated with non-toxic reference nucleic acid molecule where the non-toxic nucleic acid molecule has been validated as non-toxic in vivo (an in vivo validated non-toxic nucleic acid molecule). Such a non-toxic nucleic acid molecule can for example be compound 1-1 with SEQ ID NO: 1, in particular if the nucleic acid molecule(s) that is being subjected to the assay of the invention is a nucleic acid molecule(s), such as an antisense oligonucleotide(s). The intracellular ATP biomarker may further be compared to a second reference value obtained from cells treated with a nephrotoxic nucleic acid molecule, where the nephrotoxic reference nucleic acid molecule has been validated to cause nephrotoxicity in vivo (an in vivo validated nephrotoxic reference nucleic acid molecule).

In embodiments the cell culture medium comprises between 3 and 20 ng EGF/ml culture medium, such as between 5 and 15 ng/ml, such as between 6 and 10 ng/ml, such as at least 3 ng/ml, such as at least 4 ng/ml, such as at least 5 ng/ml, such as at least 6 ng/ml, such as at least 7 ng/ml, such as at least 8 ng/ml, such as at least 9 ng/ml. In a preferred embodiment the cell culture medium comprises between 8 and 15 ng/ml. In a further preferred embodiment the cell culture medium comprises at least 10 ng EGF/ml culture medium. This is in particular relevant where ATP is used as supplementary biomarkers.

It should be recognized that the actual level of increase/decrease of the biomarker will depend on many factors including the properties of the cell culture, the density of the cell culture, the concentration of nucleic acid molecule used, and the incubation time of the nucleic acid molecules. Relevant parameters are described in the following sections.

Cell Cultures

In the examples of the present invention several cell cultures have been tested. Both primary cell cultures as well as immortalized cell cultures appear to function in the method of the invention as long as they express epidermal growth factor receptor (EGFR). For the EGFR and KIM-1 biomarkers the EGFR receptor does not necessarily need to be functional (i.e. facilitating the consumption of EGF in the medium by the cells). A functional EGF receptor is however needed if biomarkers like ATP are to be used in the present assay. The EGFR is endogenous, meaning that it is expressed by the cell.

The method of the invention may be used to determine the likely toxicity in vivo of the nucleic acid molecule(s) in model species such as rodent species such as mouse, rat or rabbit, or pig (e.g. minipig) or dog, or primates, such as monkeys (e.g. cynomolgus monkey), or may be used to determine the likely toxicity in vivo of the nucleic acid molecule(s) in humans. The inventors have found that the use of primary EGFR expressing epithelial cells or primary hepatocytes or immortalized EGFR expressing epithelial cell are predictive of the toxicity profile seen in vivo on rodent studies as well as in human clinical trials. In particular epithelia cells which express EGFR and originate from kidney, gastrointestinal tract or lung tissue or primary hepatocytes are suitable in the method of the invention. In one embodiment the epithelial cell does not originate from the eye, in particular not from the retinal pigment epithelia, in particular the cell culture is not an ARPE19 cell culture.

In one embodiment of the invention the cells express functional EGFR, in that the cells consume EGF present in the growth medium when cultured under normal conditions (without being subjected to drug or vehicle substances). The rate of EGF consumption is preferably at least 50% EGF from the medium over 72 hours, when the cells are grown under regular conditions without being subjected to drug or vehicle substances. Some cell cultures may have a higher rate of EGF consumption such as at least 50% of the EGF in the medium over 60 hours, such as at least 50% of the EGF in the medium over 48 hours. In order to measure the EGF consumption in a cell culture it is important that the medium comprises EGF.

In one embodiment cells which express EGFR can be selected from the group consisting of epithelial cell, endothelial cell, mesenchymal cells, neuroectodermal cells and hepatocytes. In particular cell cultures originating from epithelial cells or hepatocytes are used in the method of the present invention.

In one embodiment the epithelial cells can be in the form of a mammalian primary cell culture, such as a cell culture selected from the group consisting of rodent primary epithelial cells, such as mouse or rat primary epithelial cells; pig (e.g. minipig) epithelial cells, dog epithelia cells and non-human primate primary epithelial cells, such as monkey (e.g. cynomolgus monkey) or human primary epithelial cells. In another embodiment the hepatocytes can be in the form of a mammalian primary cell culture, such as a cell culture selected from the group consisting of rodent primary hepatocytes, such as mouse or rat primary hepatocytes; pig (e.g. minipig) hepatocytes, dog epithelia cells and non-human primate primary hepatocytes, such as monkey (e.g. cynomolgus monkey) or human primary hepatocytes. In a preferred embodiment the primary epithelial or hepatocyte cell culture is obtained from a rat or a human. In addition to being obtainable from various species the cell culture may also be obtained from various organs, such as epithelial cells from the gastrointestinal tract, lungs, reproductive and urinary tracts, kidney, exocrine and endocrine glands. In one embodiment the epithelial cell culture is a kidney epithelial cell culture, gastrointestinal tract epithelial cell culture or a lung epithelial cell culture. Since the present invention sets out to predict nephrotoxicity kidney epithelial cells from selected from the group consisting of proximal tubule epithelial cells, distal tubule epithelial cells and collecting duct epithelial cells are particularly relevant. Specific examples of primary cell cultures are those made from human PTEC or rat PTEC cells. In addition to epithelial cell cultures the examples of the present invention also show that other cell types expressing EGFR can be used, for example primary hepatocytes.

In another embodiment the cells expressing EGFR are cultured from an immortalized cell line. Specific examples of cell cultures obtained from immortalized cell lines are human PTEC-TERT-1, ciPTEC, CACO2, HK-2, NKi-2 or human A549 cell lines. An example of an immortalized cell line which does express EGFR, but does not have EGFR consumption is CACO2 cells.

Administering the Nucleic Acid Molecule

The nucleic acid molecule to be assessed in the method of the present invention can be administered to the cell culture by common methods known in the art, such as passive diffusion, electroporation, sonication, cell squeezing, hydrostatic pressure, nanoparticles (e.g. liposomes), magnetofection and cell penetrating peptides. Nucleic acid molecules are generally administered using transfection or through the process known as gymnosis (also known as naked delivery, see Stein et al., NAR 2010 38(1) e3 or Soifer et al., Methods Mol Biol 2012, 815: 333-46), although other administration options also can be applied. In the examples it can be seen that the prediction of the in vitro nephrotoxicity using the EGFR biomarker is independent on whether the antisense oligonucleotide is administered to the cell culture by transfection or by gymnosis. The mode of administration needs to be adapted to the properties of the cell culture. Some cell types are more prone to take oligonucleotides up by gymnosis, as demonstrated for PTEC type cell lines, whereas other cell lines are more suitable for transfection as seen for the A549 cell line. The mode of administration is therefore subject to optimization such that the best mode of administration is investigated for a particular cell culture.

In one embodiment of the invention the nucleic acid molecule is administered by gymnosis, in particular if the nucleic acid molecule is single stranded oligonucleotides such as antisense oligonucleotides or singled stranded RNAi agents. Since its discovery over 5 years ago, gymontic delivery has become a standard tool used in oligonucleotide research, and is a well-established term used in the art. Typically, gymnotic delivery of oligonucleotides utilizes a concentration of oligonucleotide of between about 1 μM and about 1000 μM, such as between about 5 μM and about 100 μM, such as between about 10 μM and about 50 μM, such as between about 20 μM and 40 μM such as about 25-35 μM. Suitably oligonucleotides may be administered to the cell culture, e.g. in PBS, to achieve a final concentration of 1-100 μM, such as 5-50 μM, such as 10 or 30 μM. One of the advantages of gymnotic delivery is that it resembles the delivery that occur in vivo, in that no additional chemicals are needed to get the oligonucleotides into the cell.

In another embodiment of the invention the nucleic acid molecule is administered by transfection, this approach is suitable both for single stranded and double stranded oligonucleotides. Transfection can be performed using standard methods known in the art, such as lipofection, cationic polymers, calcium phosphate etc. Typically, transfection utilize nucleic acid molecule concentration of between 0.5 ng and 50 ng, such as between 1 ng and 25 ng, such as between 2 ng and 15 ng, such as between about 3 ng and 10 ng. Suitably oligonucleotides may be administered to the cell culture, e.g. in PBS, to achieve a final concentration corresponding to those indicated above.

Incubation Time

The time between administration of the nucleic acid molecule and the measurement of the relevant biomarkers is the incubation time or culturing time. For an in vitro toxicity assay to be as effective as possible the readout needs to be reproducible and consistently predict compounds with potential toxicity issues. Another relevant parameter is the time it takes to conduct the assay, the quicker it can be done the higher the throughput can be, which is highly relevant if the method of the invention is used to screen large libraries of nucleic acid molecules. The incubation time is subject to optimization depending on cell culture and method of administration. In one embodiment of the invention the incubation time with the nucleic acid molecule is between 1 and 9 days such as between 2 and 8 days, 3 and 7 days, or between 4 and 6 days, in particular between 2 and 6 days or between 3 and 6 days, such as 2, 3, 4, 5, 6, 7, 8 or 9 days. The inventors have found that for the biomarkers, EGFR and Kim-1, a sufficient reproducibility can be achieved using a 2 to 6 day incubation time, in particular biomarker measurements at day 3 and day 6 after administration show good results. In one embodiment of the invention a single stranded oligonucleotide is administered to the cell culture using gymnosis in a concentration of 50 to 100 μM and incubated for 3 to 6 days and EGFR and/or KIM-1 is measured at these times.

In the case where the intracellular biomarker, ATP, is measured the incubation time the incubation time with the nucleic acid molecule is between 5 and 10 days, such as between 6 and 9, in, such as 6, 7, 8 or 9 days.

In embodiments where the administration is performed using transfection the incubation time with the nucleic acid molecule is between 1 and 4 days, such as between 2 and 3 days, such as 1, 2, 3 or 4 days. In one embodiment of the invention a nucleic acid molecule is administered to the cell culture using transfeciton in a concentration of 1 to 20 ng and incubated for 1 to 3 days and EGFR and/or KIM-1 is measured at these times.

Cell culture of mammalian cells is typically performed at or about 37° C., and may further comprise exogenous CO₂, such kept in an atmosphere of or about 5% CO₂. Cells in culture generally needs fresh medium on a regular basis such as every 2 to 4 days. If the incubation time exceeds 3 to 4 days the medium can be exchanged every 3 to 4 days. The fresh medium preferably contains a concentration of nucleic acid molecule corresponding to the concentration given a day 0, to secure a continues presence of the nucleic acid molecule during the incubation time.

One of the advantages of the present invention is the early read out of predictive toxicity biomarkers, relatively shortly after the initiation of the incubation period, and that the biomarkers used provide a reliable signal.

Screening Library of Variants to Identify Child Nucleic Acid Molecules with a Predicted Reduced Toxicity Profile In Vivo

The invention provides for a method for selecting one or more nucleic acid molecules suitable for in vivo administration to a mammal, from a library of nucleic acid molecules, said method comprising the steps of:

-   -   a) Obtaining a library of nucleic acid molecules     -   b) Administer each member of the library of nucleic acid         molecules to a cell culture expressing epidermal growth factor         receptor (EGFR), such as described in the section “cell         cultures”;     -   c) and culturing the cells in vitro for a period of time such as         described in the section “incubation time”;     -   d) measuring the amount of at least one nephrotoxicity biomarker         such as described in the sections (Prediction of in vivo         toxicity” and “complementary biomarkers”; and     -   e) selecting one or more nucleic acid molecules wherein the %         reduction in EGFR relative to a reference value is above 80%,         such as above 85%, such as above 90, such as above 95%, such as         100% or above relative to reference value.

In one embodiment of the invention the therapeutic index of the nucleic acid molecule selected in step e) is decreased when compared to a toxic reference substance or parent nucleic acid molecule.

The selected nucleic acid molecule(s) may optionally administering in vivo to the mammal to confirm that the compound does not elicit nephrotoxicity. In particular rats are highly sensitive to nephrotoxic nucleic acid molecules, and therefore a relevant species for confirming the prediction obtained using the method of the present invention. Naturally other mammalian species mentioned herein may also be relevant.

In some embodiments, the library of nucleic acid molecules is a library of antisense oligonucleotides.

In one embodiment the library of nucleic acid molecules have different nucleobase sequences, for example they may be a library of nucleic acid molecules which are designed across a target sequence (e.g. a mRNA), for example a library of antisense oligonucleotides or RNAi agents generated by a mRNA gene-walk.

In one embodiment the members of the library of nucleic acid molecules have identical nucleobase sequences in a contiguous stretch of the sequence, where the contiguous stretch is shorter than the nucleic acid molecule, with at least a subset of the molecules in the library. Such a “hot-spot” library may for example be a library of nucleic acid molecules which are designed across a target sequence of e.g 50 to 100 nucleobases in length (e.g. a hot spot on a target RNA), where the members of the library is will be overlapping along this sequence with at least 4 to 14 nucleobases, such as 5 to 12 nucleobases such as 6 to 10 nucleobases. The library may for example be a library of antisense oligonucleotides or RNAi agents identifying the oligonucleotide with the highest TI targeting the identified hot-spot.

In some embodiments, the library of nucleic acid molecules is a library of nucleic acid molecule variants (child nucleic acid molecules) of a parent nucleic acid molecule, wherein the parent nucleic acid molecule is toxic, such as nephrotoxic, and wherein step d) identifies one or more nucleic acid molecule variants which are less toxic than the parent nucleic acid molecule; wherein the nucleic acid molecule variants retaining the core nucleobase sequence of the parent nucleic acid molecule, such as an antisense oligonucleotide.

In some embodiments, the child nucleic acid molecules may be the same length as the parent nucleic acid molecule and retain the same nucleobase sequence. However, it is envisaged that, in some embodiments, the child nucleic acid molecules may be truncated, such as by the removal of a 5′ and/or 3′ terminal nucleotide, or may in some embodiments, have an additional nucleotide at the 5′ and/or 3′ end. Removal of one or more terminal high affinity nucleosides, such as a LNA nucleoside allows for the affinity of the nucleic acid molecule to the RNA target to be maintained, as the insertion of one or more LNA nucleosides into the gap region will increase the affinity to the RNA target. It is envisaged that, in some embodiments, the library of child nucleic acid molecules may comprise variants which have different flank regions, some being truncated, some having additional nucleosides, some having a sequence shifted one or two nucleosides (as measured to the RNA target), some with additional high affinity nucleosides in the flanks, so the library is a complex library of stereodefined phosphorothioate oligonucleotides with heterogeneous phosphorothioate internucleoside linkages, thereby allowing for the concurrent selection of child nucleic acid molecules which have a decreased toxicity as compared to the parent nucleic acid molecule.

The parent and child nucleic acid molecules share a common core nucleobase sequence. The common core nucleobase sequence (or contiguous nucleobase sequence) is typically at least 10 nucleobases long, such as at least 11, at least 12, at least 13, at least 14, at least 15, or at least 16 nucleobases long, and in some embodiments may be the same nucleobase sequence of the parent nucleic acid molecule. In some embodiments the parent and (at least a proportion of) the child nucleic acid molecules have the same nucleobase sequence across the length of the nucleic acid molecules. It is however envisaged that a proportion of the child nucleic acid molecules may, in some embodiments, comprise additional 5′ or 3′ nucleotides, such as an additional 1, 2 or 3 5′ or 3′ nucleotides. In addition or alternatively in some embodiments, a proportion of the child nucleic acid molecules may be truncated with regards the parent, e.g. may comprise 1, 2 or 3nt truncation at the 5′ or 3′ end. In some embodiments, additional nucleobase or truncations of the nucleobase sequence of the (proportion of) child nucleic acid molecule (s) is a single nucleobase addition or truncation. In some embodiments, the child oligonucleotides, or a proportion thereof, may be shifted by a single nucleobase, or by 2 or 3 nucleobases in comparison to the parent nucleic acid molecule when aligned to the target sequence (in effect a truncation at one end, and an addition at the other). Additional nucleotides retain complementarity with the target nucleic acid sequence.

In some embodiments the library of nucleic acid molecule variants (child nucleic acid molecules) differs from the parent nucleic acid molecule in one or more design parameters. The design parameter can be selected from the group consisting of i) presence of one or more stereodefined phosphorothioate internucleoside linkages; ii) change in gap size; iii) introduction of a gap breaker; iv) change of wing size; v) introduction of 2′ sugar modified nucleosides; and vi) change in the 2′ sugar modified nucleoside composition in the wings introducing at least two different 2′ modified nucleosides in the wings, such as LNA nucleosides and 2′ substituted nucleosides, in particular LNA and MOE. The design parameters ii), iii), iv) and vi) are in particular for antisense oligonucleotides.

In some embodiments, the nucleic acid molecule variants are are antisense oligonucleotides.

In some embodiments the antisense oligonucleotide, is a gapmer oligonucleotide.

In some embodiments, the nucleic acid molecule variants are RNAi agents.

In some embodiments, the nucleic acid molecule variants differ from the parent nucleic acid molecule by the presence of one or more stereodefined phosphorothioate internucleoside linkages. Compounds 8-2 and 8-3 as well as compounds 10-2 to 10-5 are examples of such stereodefined variant molecules, where the parent molecules are compounds 8-1 and 10-1 respectively.

In some embodiments, the antisense oligonucleotide variants are LNA oligonucleotides.

In some embodiments, the library of child antisense oligonucleotides are or comprise a population of child oligonucleotides with different gapmer designs, optionally including different mixed wing gapmer designs, gap-breaker designs, gap length and flank length.

The method of the invention may be used to identify stereodefined nucleic acid molecules with reduced in vivo toxicity (such as nephrotoxicity), in particular stereodefined antisense oligonucleotides.

The invention therefore provides for a particular method of reducing the toxicity of an antisense oligonucleotide (parent oligonucleotide) using stereodefined phosphorothioate internucleoside linkage, comprising the steps of

-   -   a) Creating a library of stereodefined oligonucleotide variants         (child oligonucleotides), retaining the core nucleobase sequence         of the parent oligonucleotide;     -   b) Screening the library created in step a) in a cell culture         expressing epidermal growth factor receptor (EGFR); and     -   c) Identifying one or more stereodefined variants present in the         library which has a reduced toxicity in the cell culture as         compared to the parent oligonucleotide.

Optionally the method is repeated (reiterative screening), for example so that the one or more stereodefined variants identified by the method is used as a parent oligonucleotide in the next round of the screening method.

In the method of the invention, each member of the library created in step b) comprises at least one stereodefined phosphorothioate internucleoside linkage which differs from parent.

The methods of the invention may further comprise an additional subsequent step of manufacturing the one or more selected nucleic acid molecule variants which have a reduced toxicity using one of the methods of the invention. In some embodiments, the subsequent manufacture is in a scale of more than 1 g, such as more than 10 g. In some embodiments, the synthesis of the oligonucleotides for in vivo or in vitro screening steps is performed at a scale of less than 1 g, such as less than 0.5 g, such as less than 0.1 g.

In some embodiments, the methods further comprise the step of determining the in vitro or in vivo potency of either the library of nucleic acid molecules, or of the one or more selected nucleic acid molecules in the library identified in step c) or e).

The invention provides a method for predicting the (e.g. likely) in vivo nephrotoxicity of an antisense oligonucleotide, such as a LNA oligonucleotide, said method comprising the steps of administering the oligonucleotide to a cell culture expressing epidermal growth factor receptor (EGFR) optionally where the medium comprises at least 4 ng/ml of epidermal growth factor (EGF), incubating the cells in the presence of the oligonucleotide, e.g. for a period of between 2-9 days, such as 2-6 days, such as 3 days, and subsequently measuring at least one biomarker of toxicity, such as those described herein, e.g. by measuring the amount of EGFR mRNA, KIM-1 mRNA or ATP levels in the cell and/or the amount of KIM-1 released into the culture media. Suitably a reduction in cellular EGFR mRNA levels or ATP levels is indicative of a nephrotoxic oligonucleotide, and elevation of KIM-1 in the culture media is indicative of a nephrotoxic oligonucleotide. In one embodiment the EGFR biomarker is measured, optionally combined with measurement of KIM-1 and/or ATP biomarkers.

The invention provides for the use of an in vitro assay to determine the (e.g. likely) neperotoxicity of a nucleic acid molecule, such as a nucleic acid molecule, such as an antisense oligonucleotide, such as an LNA oligonucleotide.

It will be recognized that, in some embodiments, the methods for predicting (or determining) the in vivo toxicity (e.g. nephrotoxicity), may be used to identify stereodefined variants of a parent oligonucleotide, where the sterodefined variants have reduced in vitro or in vivo toxicity.

Complementary Toxicity Assays

In addition to the method for predicting in vivo nephrotoxicity of a drug substance described in this application, the method may further be combined with methods for predicting other toxicities relevant to the development of a drug substance, in particular a therapeutic oligonucleotide, such as an antisense oligonucleotide.

In some embodiments, the method for predicting nephrotoxicity disclosed or claimed in the present application may be combined with a method for predicting immunotoxicity of drug substance, in particular an oligonucleotide.

One method for predicting immunotoxicity of a drug substance in particular of an oligonucleotide, comprises measuring at least one complement biomarker and/or at least one (such as at least two) cytokine biomarkers in blood samples subjected to the drug substance. In a particular embodiment immunotoxicity is predicted by measuring at least one complement biomarker and at least two cytokine biomarkers in blood samples subjected to the drug substance, in particular an oligonucleotide.

In some embodiments the method of the invention further includes or provides a method of predicting immunotoxicity comprising the steps of a) administering the drug substance, in particular an oligonucleotide, to human blood (isolated from the body); b) incubating the samples between 30 min to 8 hours; c) stop the reaction; and d) measure at least two, three, four, five of or all of the following biomarkers: i) complement biomarkers C3a and C5a, and/or ii) cytokine biomarkers interleukin 6 (IL6), interleukin 8 (IL8), tumor necrosis factor alpha (TNFa), and monocyte chemoattractant protein-1 (MCP1); wherein a mean increase above about 2 fold compared to a control in at least two of the biomarkers is indicative of in vivo immunotoxicity of the drug substance, such as the oligonucleotide. The blood sample of step a) is typically obtained from at least one healthy human subject, such as at least two or at least three healthy human subjects. Generally, the blood samples are not mixed. In some embodiments at least one of the complement biomarkers C3a and C5a is measured in combination with at least two cytokine biomarkers selected from the group consisting of interleukin 6 (IL6), interleukin 8 (IL8), tumor necrosis factor alpha (TNFa), and monocyte chemoattractant protein-1 (MCP1). In some embodiments at least cytokine biomarkers interleukin 8 (IL8), and monocyte chemoattractant protein-1 (MCP1) are measured.

In some embodiments blood samples from at least 3 donors are used. Typically the blood is obtained from healthy donors (i.e. isolated from the body). In some embodiments the measurements from the 3 different blood samples are averaged to achieve an immunotoxicity read out.

In some embodiments, the method disclosed or claimed in the present application may be combined with a method for predicting hepatotoxicity of a drug substance, in particular an oligonucleotide. A method for predicting in vivo hepatotoxicity of an oligonucleotide is described in WO2017/067970, hereby incorporated by reference. In brief one method of predicting in vivo hepatotoxicity of an oligonucleotide comprises the steps of a) administering the oligonucleotide to a population of primary mammalian hepatocyte cells (or population of hepatocytes derived from induced pluripotent stem cells) in vitro in a cell culture media; b) culturing the cells in vitro in the cell culture media for a period of time, such as between 1 and 14 days, in particular between 2 and 7 days; and c) subsequently measuring the level of lactate dehydrogenase (LDH) released into the culture media, and/or measuring the level of cellular ATP levels; wherein an increase in lactate dehydrogenase in the cell culture media, such as a 20% increase compared to a control, or a decrease in cellular ATP levels, such as a 20% decrease compared to a control, is indicative of an oligonucleotide which is, or is predicted to be hepatotoxic in vivo in a mammal. Further biomarkers that can supplement the hepatotoxicity prediction are microRNA-122 released into the culture media, where an increase in microRNA-122 in the cell culture medium is predictive of hepatotoxicity, and intracellular glutathione (GSH) levels, where a reduction in GHS levels is predictive of hepatotoxicity.

In some embodiments of the invention the method for predicting in vivo nephrotoxicity is combined with a method of predicting in vivo immunotoxicity and a method of predicting in vivo hepatotoxicity, such as the methods described above.

Pharmaceutical Composition

In a further aspect, the invention provides a nucleic acid molecule or salts thereof obtained by the method of the invention. In a further aspect the nucleic acid molecule or salts thereof obtained by the method of the invention may be formulated into a pharmaceutical composition comprising any of the aforementioned nucleic acid molecule and a pharmaceutically acceptable diluent, carrier, salt and/or adjuvant. A pharmaceutically acceptable diluent includes phosphate-buffered saline (PBS) and pharmaceutically acceptable salts include, but are not limited to, sodium and potassium salts. In some embodiments the pharmaceutically acceptable diluent is sterile phosphate buffered saline. In some embodiments the oligonucleotide is used in the pharmaceutically acceptable diluent at a concentration of 50-300 μM solution.

Suitable formulations for use in the present invention are found in Remington's Pharmaceutical Sciences, Mack Publishing Company, Philadelphia, Pa., 17th ed., 1985. For a brief review of methods for drug delivery, see, e.g., Langer (Science 249:1527-1533, 1990). WO 2007/031091 provides further suitable and preferred examples of pharmaceutically acceptable diluents, carriers and adjuvants (hereby incorporated by reference). Suitable dosages, formulations, administration routes, compositions, dosage forms, combinations with other therapeutic agents, pro-drug formulations are also provided in WO2007/031091.

Nucleic acid molecules obtained by the method of the invention may be mixed with pharmaceutically acceptable active or inert substances for the preparation of pharmaceutical compositions or formulations. Compositions and methods for the formulation of pharmaceutical compositions are dependent upon a number of criteria, including, but not limited to, route of administration, extent of disease, or dose to be administered.

These compositions may be sterilized by conventional sterilization techniques, or may be sterile filtered. The resulting aqueous solutions may be packaged for use as is, or lyophilized, the lyophilized preparation being combined with a sterile aqueous carrier prior to administration. The pH of the preparations typically will be between 3 and 11, more preferably between 5 and 9 or between 6 and 8, and most preferably between 7 and 8, such as 7 to 7.5. The resulting compositions in solid form may be packaged in multiple single dose units, each containing a fixed amount of the above-mentioned agent or agents, such as in a sealed package of tablets or capsules. The composition in solid form can also be packaged in a container for a flexible quantity, such as in a squeezable tube designed for a topically applicable cream or ointment.

The invention provides methods for treating or preventing a disease, comprising administering a therapeutically or prophylactically effective amount of a nucleic acid molecule or salts thereof obtained by the method of the invention or a pharmaceutical composition of the invention to a subject suffering from or susceptible to the disease.

The invention also relates to a nucleic acid molecule or salts thereof obtained by the method of the invention or a pharmaceutical composition as defined herein for use as a medicament.

The nucleic acid molecule or salts thereof obtained by the method of the invention or a pharmaceutical composition according to the invention is typically administered in an effective amount.

The invention also provides for the use of the nucleic acid molecule or salts thereof obtained by the method of the invention for the manufacture of a medicament for the treatment of a disorder as referred to herein, or for a method of the treatment of as a disorder as referred to herein.

Embodiments of the Invention

The following embodiments of the present invention may be used in combination with any other embodiments described herein.

-   1. An in vitro method for predicting in vivo nephrotoxicity of a     nucleic acid molecule in a mammal, said method comprising the steps     of:     -   a. culturing cells expressing epidermal growth factor receptor         (EGFR) in a suitable cell culture media;     -   b. administering the nucleic acid molecule to said cell culture;     -   c. incubating the cells for a period of time; and     -   d. subsequently measuring the EGFR mRNA level in the cells;

wherein a decrease in EGFR mRNA levels is indicative of a nucleic acid molecule which is, or is predicted to be, associated with nephrotoxicity.

-   2. The method according to embodiment 1, wherein EGFR mRNA level is     compared to a reference value obtained from cells treated with     vehicle control or a non-toxic reference nucleic acid molecule,     where the non-toxic reference nucleic acid molecule has been     validated as non-toxic in vivo. -   3. The method according to embodiment 2, wherein the non-toxic     reference nucleic acid molecule is an antisense oligonucleotide     compound consisting of CGTcagtatgcgAATc (SEQ ID NO: 1), wherein     lower case letters represent DNA units, bold upper case letters     represent beta-D-oxy-LNA units, all LNA C are 5′methyl C and all     internucleoside linkages are phosphorothioate linkage. -   4. The method according to embodiment 3, wherein a level of EGFR     mRNA below 80% relative to the vehicle control or non-toxic     reference value is predicative of nephrotoxicity of the nucleic acid     molecule. -   5. The method according to embodiment 2 to 4, wherein EGFR mRNA     level is further compared to a second reference value obtained from     cells treated with a nephrotoxic reference nucleic acid molecule,     where the nephrotoxic reference nucleic acid molecule has been     validated to cause nephrotoxicity in vivo. -   6. The method according to embodiment 5, wherein the toxic reference     nucleic acid molecule is an antisense oligonucleotide compound     consisting of GCtgtgtgagcttGG (SEQ ID NO: 4), wherein lower case     letters represent DNA units, bold upper case letters represent     beta-D-oxy-LNA units, all LNA C are 5′methyl C and all     internucleoside linkages are phosphorothioate linkage. -   7. The method according to any one of claims 1 to 6, wherein step d)     further comprises the measurement of extracellular kidney injury     molecule-1 (KIM-1) protein or intracellular mRNA levels, wherein an     increase in KIM-1 levels are indicative of a nucleic acid molecule     which is, or is predicted to be, associated with nephrotoxicity. -   8. The method according to embodiment 7, wherein a level of KIM-1     protein above 200% relative to the saline or non-toxic reference     value is predicative of nephrotoxicity of the nucleic acid molecule. -   9. The method according to embodiment 7, wherein a level of KIM-1     mRNA above 1000% relative to the saline or non-toxic reference value     is predicative of nephrotoxicity of the nucleic acid molecule -   10. The method according to embodiment 7 to 9, wherein the increase     in KIM-1 is predicative of nephrotoxicity for a nucleic acid     molecule even if the EGFR mRNA level is not decreased. -   11. The method according to any one of embodiments 1 to 10 wherein     the culture media in step     -   a) comprises at least 4 ng/ml of epidermal growth factor (EGF)         and step d) further comprises the measurement of intracellular         adenosine triphosphate (ATP) levels; wherein a decrease in         intracellular ATP levels is indicative of a drug substance which         is, or is predicted to be, associated with nephrotoxicity. -   12. The method according to embodiment 11, wherein a level of     intracellular ATP below 80% relative to the saline or non-toxic     reference value is predicative of nephrotoxicity of the drug     substance. -   13. The method according to any one of embodiment 1 to 12, wherein     the cells expressing EGFR is selected from the group consisting of     epithelial cell, endothelial cell and mesenchymal cells,     neuroectodermal cells. -   14. The method according to any one of embodiment 1 to 13, wherein     the cells expressing EGFR is an epithelial cell culture. -   15. The method according to embodiment 13 or 14, wherein the cells     are in the form of a primary cell culture selected from the group     consisting of rodent primary cells, such as mouse or rat primary     cells; pig (e.g. minipig) cells and primate primary cells, such as     monkey (e.g. cynomolgus monkey), human primary cells. -   16. The method according to embodiment 15, wherein the primary cell     culture is obtained from a rat or a human epithelial cells. -   17. The method according to any one of embodiments 14 to 16, wherein     the epithelial cell culture is a kidney epithelial cell culture,     gastrointestinal tract epithelial cell culture or a lung epithelial     cell culture. -   18. The method according to embodiment 17, wherein the kidney     epithelial cell is selected from the group consisting of proximal     tubule epithelial cells, distal tubule epithelial cells and     collecting duct epithelial cells. -   19. The method according to any one of claim 17 or 18, wherein the     cell culture is made from human PTEC or rat PTEC cells. -   20. The method according to any one of claims 1 to 14 or 17 or 18,     wherein the cells expressing EGFR are cultured from an immortalized     cell line. -   21. The method according to embodiment 20, wherein cell culture is     obtained from the group consisting of human PTEC-TERT-1, ciPTEC,     CACO2, HK-2, NKi-2 or human A549 cell lines. -   22. The method according to any one of claims 1 to 21, wherein the     cell culture media contains at between 5 and 15 ng/ml, such as     between 8 and 15 ng/ml of epidermal growth factor (EGF), such as     around 10 ng/ml. -   23. The method according to any one of claims 1 to 21, wherein the     period of incubation with the nucleic acid molecule is between 2 and     6 days, such as around 3 days. -   24. The method according to any one of claims 1 to 23, wherein the     nucleic acid molecule is selected from a RNAi agent, an antisense     oligonucleotide or an aptamer. -   25. The method according to any one of claims 1 to 24, wherein the     nucleic acid molecule is administered to the cell culture in the     presence of a transfection agent. -   26. The method according to any one of claims 1 to 23, wherein the     nucleic acid molecule, in particular a single stranded     oligonucleotide, is administered to the cell culture in the absence     of a transfection agent, i.e. by the process referred to as     gymnosis. -   27. The method according to any one of claims 1 to 26, wherein the     nucleic acid molecule comprises one or more 2′ sugar modified     nucleosides. -   28. The method according to embodiment 27, wherein the one or more     2′ sugar modified nucleoside is independently selected from the     group consisting of 2′-O-alkyl-RNA, 2′-O-methyl-RNA, 2′-alkoxy-RNA,     2′-O-methoxyethyl-RNA, 2′-amino-DNA, 2′-fluoro-DNA, arabino nucleic     acid (ANA), 2′-fluoro-ANA and LNA nucleosides. -   29. The method according to embodiment 27 or 28, wherein the one or     more 2′ sugar modified nucleoside is a LNA nucleoside. -   30. The method according to embodiment 28 or 29, wherein the LNA     nucleoside is selected from beta-D-oxy-LNA, alpha-L-oxy-LNA,     beta-D-amino-LNA, alpha-L-amino-LNA, beta-D-thio-LNA,     alpha-L-thio-LNA, (S)cET, (R)cET, beta-D-ENA or alpha-L-ENA -   31. The method according to any one of claims 1 to 30, wherein the     nucleic acid molecule comprises at least one modified     internucleoside linkage. -   32. The method according to embodiment 31, wherein the     internucleoside linkages within the contiguous nucleotide sequence     are phosphorothioate internucleoside linkages. -   33. The method according to any one of claims 1 to 32, wherein the     nucleic acid molecule is an antisense oligonucleotide capable of     recruiting RNase H. -   34. The method according to embodiment 33, wherein the antisense     oligonucleotide is a gapmer. -   35. The method according embodiment 33 or 34, wherein the antisense     oligonucleotide is a gapmer of formula 5′-F-G-F′-3′, where region F     and F′ independently comprise 1-7 modified nucleosides and G is a     region between 6 and 16 nucleosides which are capable of recruiting     RNaseH. -   36. The method according to any one of claims 1 to 35, wherein the     in vivo nephrotoxicity is acute kidney injury and/or tubular     degradation. -   37. A method for selecting one or more nucleic acid molecules for in     vivo administration to a mammal, from a library of nucleic acid     molecules, said method comprising the steps of     -   a. obtaining a library of nucleic acid molecules;     -   b. administering each member of the library of nucleic acid         molecules to a cell culture expressing epidermal growth factor         receptor (EGFR), such as per any one of claims 13 to 22;     -   c. culturing the cells in vitro for a period of time, such as         per embodiment;     -   d. measuring the amount of intracellular EGFR mRNA for each         nucleic acid molecule, such as per any one of the claims 1 to         12; and     -   e. selecting one or more nucleic acid molecules wherein %         reduction in EGFR relative to a reference value is above 80%. -   38. The method according to embodiment 37, wherein the therapeutic     index of the selected nucleic acid molecule is decreased when     compared to a toxic reference substance or parent nucleic acid     molecule. -   39. The method according to embodiment 37 or 38, wherein the library     of nucleic acid molecules is a library of nucleic acid molecules as     per any one of claims 25 to 35. -   40. The method according to any one of claims 37 to 39, wherein the     library of nucleic acid molecules is a library of antisense     oligonucleotides. -   41. The method according to any one of claims 37 to 40, wherein the     library of nucleic acid molecules is a library of nucleic acid     molecule variants (child nucleic acid molecules) of a parent nucleic     acid molecule, wherein the parent nucleic acid molecule is toxic,     such as nephrotoxic, and wherein step d) identifies one or more     nucleic acid molecule variants which are less toxic than the parent     nucleic acid molecule; wherein the nucleic acid molecule variants     retain the nucleobase sequence of the parent nucleic acid molecule. -   42. The method according to any one of claims 37 to 41, wherein the     library of nucleic acid molecule variants comprises a population of     child nucleic acid molecules which differ by virtue of the design     from the parent nucleic acid molecule. -   43. The method according to embodiment 37 to 42, wherein the nucleic     acid molecule variants are antisense oligonucleotides and differ     from the parent antisense oligonucleotide in one or more design     parameters selected from the group consisting of     -   i. presence of one or more stereodefined phosphorothioate         internucleoside linkages;     -   ii. change in gap size;     -   iii. introduction of a gap breaker;     -   iv. change of wing size;     -   v. change in 2′ sugar modified nucleosides in the wings; and     -   vi. mixed wing gapmers with at least two different 2′ modified         nucleosides in the wings, such as LNA nucleosides and 2′         substituted nucleosides, in particular MOE. -   44. The method according to embodiment 37 to 43, wherein the     selection one or more drug substances for in vivo administration to     a mammal is further based on results from an in vitro immunotoxicity     assay and/or an in vitro hepatotoxicity assay which are suitable for     predicting in vivo immunotoxicity and/or in vivo hepatotoxicity. -   45. A nucleic acid molecule obtained by the method according to any     one of claims 37 to 43. -   46. A pharmaceutical composition comprising the nucleic acid     molecule of embodiment 44 and a pharmaceutically acceptable diluent,     solvent, carrier, salt and/or adjuvant. -   47. The nucleic acid molecule of embodiment 44 or the pharmaceutical     composition of embodiment 46 for use in a medicine.

EXAMPLES Methods and Materials Compounds

Table 1 list of oligonucleotides used in the examples

SEQ In vivo Comp ID nephro- ref Target Compound 5′ → 3′ NO toxicity  1-1 Scramble CGTcagtatgcgAATc  1 innocuous  2-1 PCSK9 AATgctacaaaaCCCA  2 low  3-1 PCSK9 TGCtacaaaacCCA  3 medium  4-1 PCSK9 GCtgtgtgagcttGG  4 high  5-1 Myd88 TAAggcaatcaagGTA  5 medium  6-1 Myd88 CAAaggaaacacaCAT  6 innocuous  7-1 Myd88 CAAatgctgaaacTAT  7 innocuous  8-1 Myd88 ACTgctttccactCTG  8 high  8-2 Myd88 ACTgc_(s)tttc_(s)cac_(s)tCTG  8 n.d  8-3 Myd88 ACTgc_(r)tttc_(r)cac_(r)tCTG  8 n.d  9-1 Myd88 GCCtcccagttccTTT  9 low/medium 10-1 Myd88 CACattccttgctCTG 10 medium 10-2 Myd88 CACatt_(s)cctt_(s)gct_(s)CT_(s)G 10 n.d 10-3 Myd88 CACatt_(r)cctt_(r)gct_(r)CT_(r)G 10 n.d 10-4 Myd88 CACatt_(s)c_(s)ctt_(s)g_(s)ctCTG 10 n.d 10-5 Myd88 CACatt_(r)c_(r)ctt_(r)g_(r)ctCTG 10 n.d 11-1 Myd88 TGCtcaacatcAAG 11 medium 12-1 Myd88 TTAcacttgacCCA 12 high 13-1 Myd88 TTTacacttgaCCC 13 medium 14-1 Myd88 GTCagaaacaaccACC 14 high 15-1 BCL11A CTAtgtgttccTGT 15 medium/high 16-1 BCL11A CGTttgtgctcgaTAA 16 medium/high 17-1 BCL11A CGTttgtgctcgATA 17 high 18-1 BCL11A ATTgcattgtttcCGT 18 low 19-1 BCL11A CATtgcattgtttCCG 19 low/medium 19-2 BCL11A CATtgcattgttTCCG 19 high 20-1 SGLT2

catgagct

20 low/medium n.d. = not determined

For the compounds lower case letters represent DNA units, upper case letters represent beta-D-oxy-LNA units. All LNA C units are 5′ methyl C and all internucleoside linkages are phosphorothioate linkage. Rp stereodefined phosphorothioate linkage are indicated by subscript r. Sp stereodefined phosphorothioate linkage are indicated by subscript s. Bold, italic lower case letters represent MOE units. In compound 20-1 all C units (DNA and MOE) are 5′ methyl C. The SEQ ID NO refers to the nucleobase sequence of the compound.

Measuring In Vivo Nephrotoxicity

Purpose bred Wistar Han Crl:WI(Han) male rats obtained from Charles River Laboratories at 7 to 8 weeks of age were divided into groups of 4 (table 1, exp. A) or 8 (table 1, exp. B) based on body weight and acclimatized for at least 5 days before dosing. The animals were housed under standard environmental conditions (22±2° C., relative humidity 50±20%, a light/dark cycle 12 h/12 h, pelleted food and water ad libitum), were offered enriched environment in an AAALAC accredited facility and were regularly and carefully monitored. All procedures were in accordance with the respective local regulations and according to the animal permissions granted by the Institutional Animal Care and Use Committee. Test compounds were formulated in isotonic sterile saline, sterile filtered (0.22 μm), and dosed at 40 mg/kg on days 1 and 8 (2.5 mL/kg) in the intrascapular region. Control group animals received saline as vehicle control. On day 15 animals were orally administered tap water (10 mL/kg), and urine was collected on ice for 6 hours in metabolic cages. Urine protein levels (Aution Max AX-4280) and urinary renal injury biomarkers were measured (Multiplex MAP Rat Kidney Toxicity Magnetic Bead Panel 2). On day 15 the rats were sacrificed by an intraperitoneal injection of pentobarbital and exsanguinated. Kidney cortex samples were collected and fixed by immersion in 10% neutral buffered formalin, embedded in paraffin, sectioned to 5 μm and stained with hematoxylin and eosin (H&). The H&E sections were then scanned at 20× magnification using an Aperio ScanScope AT (Leica Biosystems) scanner and pictures were then captured via ImageScope software from the scanned images. One or more of the following parameters were assessed kidney weight, serum creatinine, urine protein, KIM-1 protein in urine, KIM-1 mRNA, kidney degeneration/regeneration and relative tubulotoxicity grade.

Cell Cultures Human Primary Proximal Tubule Epithelial Cells (PTEC) Cell Culture

Primary PTEC (Science Cell Research Labotories catalog #4100) were cultured according to the manufacturer's instructions in PTEC medium [DMEM/F12 without phenol red (ThermoFisher Scientific 11039021) containing 1% Penicillin-Streptomycin solution (ThermoFisher Scientific 15140122), 10 mM HEPES (ThermoFisher Scientific 15630056), 5 ug/ml insulin and 5 ug/ml transferrin and 8.65 ng/ml sodium selenite (all from a 100× concentrated stock solution, ThermoFisher Scientific 41400045), 100 nM hydrocortisone (Sigma H6909), 3.5 ug/ml ascorbic acid (Sigma A4403), 25 ng/ml prostaglandin E1 (Sigma P5516), 3.25 pg/ml triiodo-L-thyronine (Sigma T6397), 10 ng/ml human recombinant epidermal growth factor (EGF, R&D Systems 236-EG-200), and 100 μg/ml Geneticin (G418 sulfate, ThermoFisher Scientific 10131027)].

Prior to treatment with oligonucleotides the primary PTEC cells were seeded into collagen I-coated 96-well plates (Corning, 356407) at a density of 40 000 and 20 000 cells/well respectively in PTEC medium and grown until confluence.

Human PTEC-TERT1 Cell Culture

PTEC-TERT1 (Evercyte GmbH, Austria) were cultured according to the manufacturer's instructions in PTEC medium [DMEM/F12 without phenol red (ThermoFisher Scientific 11039021) containing 1% Penicillin-Streptomycin solution (ThermoFisher Scientific 15140122), 10 mM HEPES (ThermoFisher Scientific 15630056), 5 ug/ml insulin and 5 ug/ml transferrin and 8.65 ng/ml sodium selenite (all from a 100× concentrated stock solution, ThermoFisher Scientific 41400045), 100 nM hydrocortisone (Sigma H6909), 3.5 ug/ml ascorbic acid (Sigma A4403), 25 ng/ml prostaglandin E1 (Sigma P5516), 3.25 pg/ml triiodo-L-thyronine (Sigma T6397), 10 ng/ml human recombinant epidermal growth factor (EGF, R&D Systems 236-EG-200), and 100 μg/ml Geneticin (G418 sulfate, ThermoFisher Scientific 10131027)].

Prior to treatment with oligonucleotides the PTEC-TERT1 were seeded into collagen I-coated 96-well plates (Corning, 356407) at a density of 40 000 and 20 000 cells/well respectively in PTEC medium and grown until confluence.

Rat Primary Proximal Tubule Epithelial Cells (PTEC) Cell Culture

Proximal renal tubule epithelial cells were prepared by a simplified procedure of that described by Bruce et al, Methods Mol Biol 1001, 53-64 (2013). Kidneys were removed from one anesthetized male Wistar rat (age: 10-18 weeks) and were washed in cold 1× concentrated Hanks balanced salt solution (HBSS, ThermoFisher Scientific 14065049). The organs were decapsulated, and the outer stripes of the kidney cortex without medulla were cut into 1 to 2 mm³ pieces. Tissue pieces were digested in 25 ml of HBSS containing 2 mg/ml collagenase A (Roche 10103586001) and 10 ug/ml DNAse I (Roche 10104159001) at 37° C. for 60 min. with continuous gentle shaking. The reaction was stopped by addition of 25 ml of ice-cold HBSS containing 2% bovine serum albumin (BSA, Fraction V, Roche 10735086001). Dissociated tissue was filtered consecutively first through a 200 μm cell strainer (pluriSelect 43-50200) and subsequently through a 100 um cell strainer (pluriSelect 43-50100); the filtrate containing single cells and tubule fragments was washed and centrifuged three times (100 g) in HBSS solution without MgCl2 and CaCl2 (HBSS−/−, ThermoFisher Scientific 14175053). The sediment was resuspended in 25 ml HBSS−/− and mixed with 25 ml of 30% OptiPrep solution [mixture of 5 volumes of 60% OptiPrep density gradient media (Sigma D1556), 4 volumes of H2O sterile, and 1 volume of 10× concentrated phosphate buffered saline without MgCl2 and CaCl2 (PBS−/− ThermoFisher Scientific 14200-067) to obtain a suspension of cells and tubular fragments in 15% OptiPrep. The suspension was centrifuged (800 g, at room temperature for 20 min). The cell band in the upper third of the tube was harvested; cells in the sediment at the bottom of the tube were discarded. Harvested cells were washed and centrifuged three times (400 g, at room temperature for 5 min.) in rat PTEC medium [1 volume DMEM (ThermoFisher Scientific 11966025), 1 volume Ham's F-12 nutrient mix (ThermoFisher Scientific 21765029), 2% fetal bovine serum (FBS, ThermoFisher Scientific 16000044), 1% Penicillin-Streptomycin solution (ThermoFisher Scientific 15140122), 10 mM HEPES (ThermoFisher Scientific 15630056), 5 ug/ml insulin and 5 ug/ml transferrin and 8.65 ng/ml sodium selenite (all from a 100× concentrated stock solution, ThermoFisher Scientific 41400045), 100 nM hydrocortisone (Sigma H6909), 3.5 ug/ml ascorbic acid (Sigma A4403), 25 ng/ml prostaglandin E1 (Sigma P5516), 3.25 pg/ml triiodo-L-thyronine (Sigma T6397), and 10 ng/ml rat recombinant epidermal growth factor (EGF, R&D Systems 3214-EG-100/CF)]. After the final centrifugation step, the cell preparation was resuspended in 50 ml of rat PTEC medium and distributed into three collagen I-coated 150 cm² cell culture flasks (Corning 354486) followed by incubation for 4 days with a change of medium after the first 2 days.

Prior to treatment with oligonucleotides the expanded rat PTEC cells were harvested from the culture flasks by detachment with trypsin-EDTA solution (ThermoFisher Scientific 25200056), washed in rat PTEC medium and seeded into collagen I-coated 96 well plates (Corning, 356407) at a density of 36 000 cells/well in rat PTEC medium for growth until confluence.

CACO2 (Human Epithelial Colorectal Adenocarcinoma Cells)

CACO2 (ATCC, HTB-37) were cultivated according to the manufacturer's instructions in CACO2 medium [DMEM/F12-Glutamax, non-essential amino acid (1%), penicillin/streptomycin (1%) (Gibco, 31331-028)(Gibco, 11140-035)(Gibco: 15140-122), 20% FBS (Gibco, 16000-044] for 2 passages then switched to CACO2 medium containing 10% FBS.

Prior to treatment with oligonucleotides the CACO2 cells were seeded into 96-well plates at 10 000 cells per well and grown until confluence.

A549 Cells (Adenocarcinomic Human Alveolar Basal Epithelial Cells)

A549 cells (ATCC CCL-185) were cultivated according to the manufacturer's instructions in A549 medium [F-12K Nut Mix (Gibco, 21127-022), 1% penicillin/streptomycin (Gibco: 15140-122), 10% FBS (Gibco 16000-044)].

Prior to treatment with oligonucleotides the A549 cells were seeded in 96 well plates at 3000 cells per well in A549 regular medium and grown until 60% confluence.

For lipofection, cells were transfected with 1 or 10 ng of oligonucleotide using lipofectamin (Invitrogen, 11668-019) according to the manufacturer's instructions. After 24 hours the medium was changed for A549 regular medium containing 10 ng/ml EGF and 2% FCS. After 72 hours the cells were harvested and EGFR mRNA was measured and the supernatant was stored at −20° C. for KIM-1 analysis.

For gymnosis the cells were grown to confluence and subjected to the gymnosis protocol below.

Oligonucleotide Treatment Using Gymnosis

Oligonucleotides were dissolved in PBS and added to the cell culture at the given concentration, such as 10, 30 or 100 μM. The total volume of each well was 100 μl. PBS served as vehicle control.

When intracellular ATP was to be analyzed following the oligonucleotide treatment the medium was changed every 3 days including addition of the same concentration of oligonucleotide as day 0.

When extra cellular markers, like KIM-1, were analyzed following the oligonucleotide treatment the medium was collected and stored at −20° C. until further analysis. Cells that were grown beyond 3 days of the first oligonucleotide treatment had the medium collected and replaced every 3 days incl. fresh oligonucleotide. The collected medium was stored at −20° C.

ATP Assay

For the determination of intracellular ATP levels the CellTiter-Glo® Luminescent Cell Viability Assay (G7571, Promega Corporation, Madison Wis., USA) was used according to the manufacturers instructions. Each sample was tested in triplicate. Unless indicated otherwise the intracellular ATP levels were measured at day 9 after oligonucleotide treatment. A decrease in ATP levels below 80% in relation to vehicle was considered as predictive for nephrotoxicity.

EGFR and PCSK9 mRNA Assay

Cells were collected by replacing culture medium with 100 μl/well of 1× RNA lysis mixture (QuantiGene® Sample Processing Kit, QS0101). RNA lysis mixtures were kept at −80° C. until analysis. 20 μl of lysates were mixed with an mRNA-capture magnetic beads sets (for human cells Panomics QuantiGene® Plex Set #12871 and for rat cells Panomics QuantiGene® Plex Set #31357), incubated overnight, processed for branched DNA amplification and analyzed according to the manufacturer's instructions (Panomics QuantiGene® Plex Assay kit, QP1015). The PPIB probe was used as housekeeping gene for normalization. Average Fluoresence Intensity (FI) and standard deviation of 3 biological replicates were calculated and normalized on vehicle control. A decrease in EGFR mRNA levels below 80%, preferably below 75%, in relation to vehicle was considered as predictive for nephrotoxicity.

KIM-1 Assay

For analysis of human and rat KIM-1, cell supernatants were thawed on ice, diluted 1:2 and 1:10 in sample dilution buffer (BioRad catalog #M60-009RDPD) and analyzed by Luminex-based ELISA using human KIM-1 beads (Human Kidney Injury panel 4, Millipore HKI4MAG-99K-KIM1) or rat Kim-1 beads (Milliplex Rat Kidney toxicity RKTX1MAG-37K-Kim1) followed by analysis using the Bio-Plex® 200 Systems (BioRad) according to the manufacturer's instructions. Data are reported as mean concentrations and standard deviations of triplicate wells. An increase of KIM-1 protein levels above 200% in relation to vehicle was considered as predictive for nephrotoxicity.

KIM-1 mRNA levels were measured according to the same procedure as the EGFR mRNA levels. In rats Panomics QuantiGene® Plex Set #31357 was used, where HAVCR1 corresponds to KIM-1. An increase of KIM-1 mRNA levels above 1000% in relation to vehicle was considered as predictive for nephrotoxicity

Example 1 Morphological Changes of Cell Cultures Upon Oligonucleotide Treatment

The present example evaluates the effect on the morphology of a cell culture following oligonucleotide treatment.

PTEC-TERT1 cells were cultures as described in the “Materials and methods” section. To mimic the physiological exposure of renal tubules to circulating naked oligonucleotide (i.e. without assistance of delivery technology, herein termed gymnosis or gymnotic delivery), confluent monolayers of PTEC-TERT1 cells were exposed to an aqueous solution of 100 μM oligonucleotide. The medium was replaced every three days including 100 μM fresh oligonucleotide in the fresh medium.

After 7 days of treatment the morphological alterations in the treated cell cultures were investigated under bright field microscopy. FIG. 1 shows that PTEC-TERT1 cells treated with oligonucleotide compound 1-1 (innocuous in vivo) did not show any morphological changes compared to saline treated cells. Cells treated with oligonucleotide compound 3-1 (medium in vivo tox) formed irregular domes and vacuoles whereas PTEC-TERT1 cells treated with oligonucleotide compound 4-1 (high in vivo tox) adopted a flattened and stable appearance. Both the toxic compounds show morphological changes, however the less toxic compound 3-1 produce more significant morphological changes than the highly toxic compound 4-1.

In conclusion toxic oligonucleotides affect the morphology, the severity of the toxicity can however not be predicted using morphological changes.

Example 2 PCSK9 Targeting Oligonucleotides and Their Effects on EGFR mRNA Expression in PTEC-TERT1 Cells

The present example evaluates the effect on the biomarker, EGFR, in cells exposed to oligonucleotides in a time course from 8 hours to 6 days. The effect on the target nucleic acid, PCSK9 was also analyzed to show efficacy of the compounds.

The immortalized PTEC-TERT-1 cell line was cultured according to the conditions described in the “Materials and methods” section. At confluence the cells were treated with oligonucleotide as described in the “Materials and methods” section, in concentrations of 100 μM.

The EGFR mRNA level and PCSK9 mRNA level in the cells was measured according to the assay as described in the “Materials and methods” section.

The results are shown in tables 2 and 3 below and represent the average of three identical treatments.

TABLE 2 EGFR mRNA concentrations as % of saline after oligonucleotide treatment for the indicated time 8 h 24 h 48 h 72 h Day 6 In vivo tox Comp # EGFR SD EGFR SD EGFR SD EGFR SD EGFR SD saline 100 12 100 29 100 4 100 10 100 11 Innocuous 1-1 98 5 99 6 99 6 97 8 106 5 low 2-1 98 9 100 5 116 3 122 12 129 8 Medium 3-1 90 7 94 6 89 5 89 11 74 5 high 4-1 96 13 76 3 73 4 56 2 46 5

TABLE 3 PCSK9 mRNA concentrations as % of saline after oligonucleotide treatment for the indicated time 8 h 24 h 48 h 72 h Day 6 In vivo tox Comp # PCSK9 SD PCSK9 SD PCSK9 SD PCSK9 SD PCSK9 SD saline 100 15 100 3.3 100 5 100 12 100 4 Innocuous 1-1 93 1.4 102 1.4 105 2.4 126 14.6 90 11.2 low 2-1 29 0.2 3.5 1.2 1.8 0.3 1.1 0.2 0.7 0.3 Medium 3-1 40 1.6 6.7 1.6 2.5 0.3 0.5 0.2 0.5 0.2 high 4-1 66 4.0 32 1.2 10 0.8 3.5 1.3 1.9 1.1

From this it can be seen that already after 48 hours the highly toxic oligonucleotide (comp 4-1) starts to down regulate EGFR, whereas the medium toxic compound (comp 3-1) shows effects on EGFR down regulation after 6 days. The compounds targeting PCSK9 (comp 2-1, 3-1 and 4-1) all show effective knock down of PCSK9 after 24 hours. The low toxic compound 2-1 actually appears to be the most effective in down regulating PCSK9, so the down regulation of PCSK9 does not appear to contribute to the toxicity of the oligonucleotides.

A further investigation of the compounds that down regulate EFGR (comp 3-1 and 4-1) showed that these oligonucleotides contained only one mismatch to the EGFR premRNA, whereas the innocuous compounds did not show any significant match (complementarity) to the EGFR mRNA. The down regulation of the EGFR mRNA could therefore theoretically be due to off-target effects, we do however not believe this is the case based on the observations found in Example 3 below.

Example 3 PCSK9, MYD88 and Bcl11A Targeting Oligonucleotide Effects on Extracellular

The present example evaluates whether the findings in example 2 can be reproduced for a larger set of oligonucleotides directed to other targets. In the same study the biomarker KIM-1, EGF and ATP was measured as well.

The immortalized PTEC-TERT-1 cell line was cultured according to the conditions described in the “Materials and methods” section. At confluence the cells were treated with oligonucleotide as described in the “Materials and methods” section, in concentrations of 10, 30 or 100 μM.

For EGFR and KIM-1 measurements were performed at day 6. EGFR mRNA and KIM-1 protein levels were measured according to the assays described in the “Materials and methods” section.

The results are shown in tables 4 below, and represent the average of three identical treatments.

TABLE 4 EGFR mRNA level in the cells and KIM-1 levels in culture media at day 6 after oligonucleotide treatment and intracellular ATP levels was measured at day 9 after oligonucleotide treatment. In vivo Day 6 Day 6 Day 9 grade Comp Conc EGFR KIM-1 ATP of toxicity # μM % saline SD % saline SD % saline SD High 4-1 30 60 6.5 43 6.4 n.d 100 44 2.0 1 2.6 n.d. Innocuous 6-1 10 105 1.6 140 13 93 4 30 102 3.6 150 6 99 3 100 115 3.0 122 8 101 3 Innocuous 7-1 10 98 9.9 159 4 113 7 30 98 17.0 127 3 114 6 100 97 9.7 120 6 107 1 High 8-1 10 44 4.2 78 29 59 3 30 27 0.3 63 1 47 7 100 21 1.0 54 1 43 1 Medium 9-1 10 64 0.6 151 7 99 2 30 53 8.8 129 8 101 2 100 50 0.7 116 29 103 4 Medium 10-1  10 80 5.9 123 17 87 2 30 68 6.2 77 1 66 6 100 66 7.2 65 4 60 5 Medium 11-1  10 37 0.6 149 13 136 2 30 29 11.0 111 10 135 6 100 18 0.6 82 8 119 4 High 12-1  10 102 3.8 325 37 132 2 30 104 7.9 379 20 133 1 100 94 5.2 289 26 90 4 Medium 13-1  10 115 6.2 268 46 124 10 30 115 7.6 242 51 122 5 100 114 6.6 252 17 114 2 Medium 15-1  10 68 2.5 43 3 101 2 30 59 5.2 34 3 92 0 100 65 3.3 25 2 52 2 Mild tox 18-1  10 96 1.8 188 17 121 1 30 104 10.2 193 21 112 4 100 98 10.8 181 13 105 0 Mild tox 19-1  10 86 7.6 120 11 100 2 30 76 1.4 129 24 90 2 100 64 2.3 77 15 76 1 Medium 16-1  10 91 1.4 160 10 123 1 30 75 5.2 164 15 122 1 100 72 4.4 129 16 113 0 High 19-2  10 69 3.4 75 11 67 1 30 56 5.2 57 16 54 2 100 66 8.1 28 4 40 1 High 17-1  10 77 9.1 167 20 124 1 30 64 7.9 202 4 116 2 100 64 22.2 140 23 96 1

From table 4 it can be seen that the EGFR biomarker is capable of predicting 10 out of 13 toxic compounds at the 100 μM oligonucleotide dose. Of these oligonucleotides compound 13-1 and 15-1 have two mismatches to human EGFR premRNA. Compound 13-1 does not affect the EGFR mRNA levels so two mismatches in this compound most likely results in a binding affinity that is too low to result in cleavage of the EGFR premRNA. Compounds 8-1, 9-1, 10-1, 11-1, and 16-1 all reduce the level of EGFR mRNA, none of these compounds are complementary to the human EGFR premRNA to a level where they would be expected to cleave the target (they have more than 3 mismatches to human EGFR premRNA). Consequently, the down regulation of EGFR mRNA by these compounds cannot be attributed to off-target effects and therefore establishes that EGFR mRNA is a relevant biomarker for the prediction of nephrotoxicity of oligonucleotides independent of their level of complementarity to EGFR premRNA.

KIM-1 only predicts 2 out of the 13 toxic compounds. However, these are the compounds that were not caught be the EGFR biomarker, indicating that KIM-1 can supplement the predictions made with EGFR as biomarker.

ATP as biomarker is capable of predicting 5 of the 12 toxic compounds. Consequently, the ATP biomarker can be used to supplement the EGFR biomarker.

The results are also summarized in FIG. 2.

Example 4 PCSK9 and Bcl11A Targeting Oligonucleotides and Their Effects on EGFR and KIM-1 Expression in Rat Primary PTEC Cells

The present example evaluates whether the findings in example 2 and 3 can be reproduced in a cell line from a different species.

A cell culture of primary rat PTEC cells were made and cultured according to the conditions described in the “Materials and methods” section. At confluence the cells were treated with oligonucleotide as described in the “Materials and methods” section, in concentrations of 1, 10, or 100 μM.

For EGFR and KIM-1 measurements were performed at day 3. EGFR mRNA and KIM-1 protein levels were measured according to the assays described in the “Materials and methods” section.

The results are shown in tables 5 below, and represent the average of three identical treatments.

TABLE 5 EGFR and KIM-1 levels at day 3 after oligonucleotide treatment. In vivo grade of Conc EGFR KIM-1 mRNA KIM-1 prot toxicity Comp # μM % 1-1 SD % 1-1 SD % 1-1 SD Innocuous 1-1 1 100 7.2 100 18.7 100 13.0 10 100 11.5 100 32.6 100 9.0 100 100 9.4 100 20.6 100 10.4 medium 3-1 1 67 9.0 1321 106.7 262 48.3 10 84 5.9 3622 93.4 433 101.8 100 99 17.5 2874 486.7 65 7.5 High 4-1 1 23 4.4 213 71.4 99 20.8 10 12 1.0 254 98.3 98 10.5 100 11 7.3 67 31.7 92 Medium/high 15-1 1 39 7.6 299 144.0 103 27.4 10 29 7.0 354 81.2 114 23.4 100 68 5.1 151 110.7 152 50.1 Medium/high 16-1 1 83 18.6 188 75.1 122 33.5 10 90 18.0 356 123.9 140 42.1 100 104 18.0 226 69.5 141 43.6 High 17-1 1 83 13.1 306 80.0 108 21.2 10 83 18.4 405 116.7 151 32.7 100 95 16.5 422 115.8 184 55.0 Low 18-1 1 64 5.8 423 69.6 137 22.2 10 42 11.4 556 105.9 159 22.4 100 51 12.2 526 474.7 174 51.1 Low/medium 19-1 1 53 10.5 1676 480.0 185 46.4 10 48 17.4 1991 781.4 231 72.1 100 35 14.7 1437 378.5 345 52.2 High 19-2 1 25 10.5 5139 1462.9 502 81.3 10 10 7.7 5361 1106.2 712 88.8 100 6 10.3 2367 606.9 566 149.7

Primary rat PTEC cells are quite sensitive to oligonucleotide treatment in general and it appears that doses of 100 μM oligonucleotide affect the cells to an extent where the assay becomes less predictable. To account for the sensitivity of the rat PTEC cells the data in table 5 have been normalized to the non-toxic toxic reference antisense oligonucleotide indicated as comp 1-1. Using a reduction in the EGFR level as a biomarker the assay is capable of predicting 6 out of 8 toxic compounds at the 1 μM dose (comp 3-1, 4-1 15-1, 18-1, 19-1 and 19-2). None of the compounds have below 2 mismatches to rat EGFR premRNA consequently the effects are not expected to be off-target effects.

Increases in KIM-1 levels are significantly different at the mRNA level and the protein level. For KIM-1 mRNA levels the threshold for an indication of toxicity was set at a 10 fold increase over the innocuous compound 1-1. The threshold for an indication of toxicity when measuring KIM-1 protein level was set at a 2 fold increase over the innocuous compound 1-1. With these thresholds 3 out of the 8 toxic compounds were predicted as toxic (comp 3-1, 19-1 and 19-2) indicating that KIM-1 can supplement the predictions made with EGFR as biomarker for some compounds.

From this it can be seen that the EGFR biomarker in rat primary PTEC cells can be used to predict the in vivo toxicity of oligonucleotides. The cells are however more sensitive to oligonucleotide treatment, and it is therefore recommended to perform the evaluation in relation to a non-toxic toxic reference antisense oligonucleotide and at lower oligonucleotide concentrations than for human PTEC and PTEC-TERT1 cells.

Example 5 Oligonucleotide Effects on EGFR in CACO2 Cells

In the following example it was investigated whether a cell line that does not originate from the kidney and which does not have an active EGF consumption but which does express EGFR can be used to predict nephrotoxicity of an oligonucleotide.

The immortal CACO2 cell line was cultivated as described in the “Materials and methods” section without the presence of EGF to the medium. At confluence the cells were treated with oligonucleotide using gymnosis as described in the “Materials and methods” section, in concentrations of 1, 10 or 100 μM.

The cells were harvested at day 6, and the EGFR and PCSK9 mRNA level was measured according to the assay described in the “Materials and methods” section.

The results are shown in table 6 below, and represent the average of three identical treatments.

TABLE 6 EGFR and PCSK9 mRNA levels in CACO2 cells at day 6 after oligonucleotide treatment. ATP levels after 9 days treatment. In vivo EGFR PCSK9 ATP grade Comp Conc % % % of toxicity # μM saline SD saline SD saline SD saline 0 100 4.4 100 5.2 100 5.2 Innocuous 1-1 1 74 5.9 99 5.5 108 9.0 10 71 7.0 108 9.6 98 13.3 100 83 5.4 145 5.5 93 15.4 low 2-1 1 80 7.6 39 3.2 104 9.6 10 68 1.4 10 1.3 102 14.4 100 57 4.8 3 0.1 103 10.2 Medium 3-1 1 91 2.5 37 3.0 107 10.5 10 72 5.7 9 1.3 97 4.5 100 45 1.4 2 0.1 97 9.0 High 4-1 1 86 11.4 75 16.7 102 6.8 10 36 4.6 15 2.0 100 6.7 100 15 4.9 4 0.8 82 7.3

From this it can be seen that at 10 and 100 μM oligonucleotide the nephrotoxic compounds (comp 3-1 and 4-1) can be identified using CACO2 cells. The conditions of this example does however not allow generate predictive results for ATP as a biomarker.

Example 6 Oligonucleotide Effects on EGFR in A549 Cells

In this example it was tested whether another cell line that does not originate from the kidney which do have an active EGF consumption and express EGFR can be used to predict nephrotoxicity of an oligonucleotide.

A549 were cultivated as described in the “Materials and methods” section. At confluence the cells were treated with oligonucleotide using gymnosis as described in the “Materials and methods” section, in concentrations 100 μM.

The cells were harvested at day 2 and the EGFR and PCSK9 mRNA level was measured according to the assay described in the “Materials and methods” section.

The results are shown in table 7 below, and represent the average of three identical treatments.

TABLE 7 EGFR and PCSK9 mRNA levels in A549 cells at day 2 after gymnotic oligonucleotide treatment. In vivo grade of Conc EGFR PCSK9 toxicity Comp # μM % saline SD % saline SD saline 0 100 5.7 100 0.2 Innocuous 1-1 100 97 2.5 93 3.6 Medium 3-1 100 83 1.2 0 0.9 High 4-1 100 33 5.0 1 0.2 High 8-1 100 32 5.4 145 9.7

From this it can be seen that at 100 μM oligonucleotide the highly nephrotoxic compounds (comp 4-1 and 8-1) can be identified using A549 cells and gymnotic delivery of the oligonucleotide. The medium nephrotoxic compound (comp 3-1) has reduced EGFR very close to 80% of saline which considering the short incubation time can be considered as indicative of potential toxicity.

Therefore it is concluded that P549 cells are useful in identifying nephrotoxic compounds using EGFR mRNA as biomarker and gymnosis for delivery, potentially with an incubation time of more than 2 days.

Example 7 PCSK9 Targeting Oligonucleotide Effects on EGFR in A549 Cells Using Transfection

In this example it was tested whether a cell line that is suitable for transfection could be applied in the method of predicting nephrotoxicity.

A549 were cultivated as described in the “Materials and methods” section. At after at 50-60% confluence the oligonucleotides were transfected into the cells using 0.5 μl Lipofectamin (Invitrogen, 11668-019) in 25 μl OptiMEM (GIBCO 31985062) and 1 ng oligonucleotide in the same volume OptiMEM. The cells were incubated over night at 37° C. The medium was changed using A459 regular medium+10 ng/ml EGF. 48 hours after transfection the cells were harvested and the EGFR mRNA level, PCSK9 mRNA levels and ATP levels were measured.

The results are shown in table 8 below, and represent the average of three identical treatments.

TABLE 8 EGFR, ATP and PCSK9 mRNA levels from A549 cells 48 hours after transfection with oligonucleotide In vivo EGFR PCSK9 ATP grade of Comp Conc % % % toxicity # ng saline SD saline SD saline SD saline 0 100 12.9 100 13.4 100 12.7 Innocuous 1-1 1 110 12.7 107 4.8 92 8.8 Medium 3-1 1 75 9.1 21 1.8 48 3.8 High 4-1 1 62 6.4 31 8.3 34 10.6 High 8-1 1 82 5.1 153 7.4 36 20.2

These data show that EGFR can also be used as a biomarker for nephrotoxicity in transfected epithelial cells. The nephrotoxic oligonucleotides (comp 3-1 and 4-1) were predicted as being nephrotoxic at only 1 ng of oligonucleotide after just 48 hours incubation. The ATP biomarker supports these data nicely.

The data also show that PCSK9 was knocked down by the oligonucleotides targeting PCSK9 (comp 3-1 and 4-1), and not by the non-targeting compounds 1-1 and 8-1.

Example 8 PCSK9 and MYD88 Targeting Oligonucleotide Effects on EGFR in A549 Cells Using Transfection

In this example it was tested whether a cell line that is suitable for transfection could be applied in the method of predicting nephrotoxicity.

A549 were cultivated as described in the “Materials and methods” section. At after at 50-60% confluence the oligonucleotides were transfected into the cells using 0.5 μl Lipofectamin (Invitrogen, 11668-019) in 25 μl OptiMEM (GIBCO 31985062) and 1 ng oligonucleotide in the same volume OptiMEM. The oligonucleotides comp 1-1 and 2-1 was transfected using 10 ng. The cells were incubated over night at 37° C. The medium was changed using A459 regular medium+10 ng/ml EGF. 48 hours after transfection the cells were harvested and the EGFR mRNA level was measured.

The results are shown in table 9 below, and represent the average of three identical treatments.

TABLE 9 EGFR mRNA levels from A549 cells 48 hours after transfection with oligonucleotide In vivo grade of Conc EGFR KIM-1 toxicity Comp # ng % saline SD % saline SD saline 0 100 0.3 100 4.3 Innocuous  1-1 10 109 11.6 90 6.0 low  2-1 10 100 6.9 68 1.6 Innocuous  6-1 1 106 8.7 77 12.0 High  4-1 1 71 3.9 84 12.0 High  8-1 1 65 3.6 84 4.5 Low/medium  9-1 1 66 4.2 91 8.0 Medium 10-1 1 73 5.3 78 3.3 Medium 11-1 1 63 2.3 90 2.9 High 12-1 1 124 4.6 92 2.6 Medium 13-1 1 120 4.3 87 7.6

Of the oligonucleotides tested in this example the EGFR biomarker identified 5 out of 7 nephrotoxic compounds (comp 4-1, 8-1, 9-1, 10-1 and 11-1). As in Example 3 comp 12-1 and 13-1 was not predicted as nephrotoxic using the EGFR biomarker or the KIM-1 biomarker.

The EGFR biomarker appears to be a good biomarker in a transfection based assay which has the advantage that short incubation times and small amounts of oligonucleotide is needed.

Example 9 Effect on ATP as Biomarker when EGFR is Blocked

In example 7 it was shown that in CACO2 cells ATP was not predictable as biomarker. CACO2 cell proliferation and survival do not dependent on EGF in the culture conditions as described here. The present example set out to identify whether blocking EGFR on the cell line used for the nephrotoxicity assay of the invention affects the ATP biomarker.

Erlotinib, a small molecule inhibitor of EGFR kinase activity was used in the present assay at 5 μM. Intracellular ATP levels were measured in confluent PTEC-TERT1 after 9 days exposure to 100 μM oligonucleotide along with 10 ng/ml of EGF in the medium with and without erlotinib. The results are shown in table 10, and represent the average of three identical treatments.

TABLE 10 Effect on intracellular ATP of oligonucleotides in the presence of erlotinib No erlotinib 5 μM erlotinib In vivo grade ATP ATP of toxicity Comp# % Saline SD % Saline SD Innocuous 1-1 108.61 5.43 95.54 3.02 low 2-1 107.67 2.93 84.31 1.07 Innocuous 6-1 102.45 2.36 104.16 2.82 Medium 3-1 87.67 2.19 89.59 4.74 High 5-1 82.90 3.40 89.58 4.61 High 4-1 65.71 3.20 94.44 4.74 High 8-1 50.28 0.20 97.47 2.46

These data show that the ATP profile of innocuous and toxic oligonucleotides was undistinguishable in cells where EGFR was inactivated using erlotinib. This is a strong indication that EGFR expression is need to be functional in cells when assessing the nephrotoxicity profile of oligonucleotides in cell based assays.

Example 10 Investigation of EGF Concentrations in the Medium when Using ATP as Biomarker

As shown in example 9 it is likely that a functional EGF receptor is needed on the cells when ATP is used as biomarker. The present example evaluates the effect of the EGF concentration in the culture medium on the intracellular ATP levels as well as on the target knockdown by the oligonucleotides.

Intracellular ATP level was measured in confluent PTEC-TERT1 after 9 days exposure to 100 μM oligonucleotide along with 0, 1, 3, 10, 30 and 100 ng/ml of EGF in the medium. The results are shown in table 11, and represent the average of three identical treatments.

TABLE 11 Intracellular ATP as % of saline with varying levels of EGF in the medium EGF ng/ml 0 1 3 10 30 90 Comp # ATP SD ATP SD ATP SD ATP SD ATP SD ATP SD saline 100 4 100 5 100 6 100 4 100 4 100 11 2-1 85 3 89 6 104 3 92 6 86 2 78 3 3-1 101 1 106 3 101 5 63 2 59 0 56 2 4-1 88 3 95 3 62 2 29 1 30 1 30 1

These results show that when applying oligonucleotide to PTEC-TERT1 cells the effect on the intracellular ATP levels is dependent on the EGF concentration in the medium, whereas the target knockdown is unaffected by the EGF levels in the medium. At 10 ng/ml of EGF in the medium the toxicity of the oligonucleotide compounds can be differentiated nicely, whereas below 3 ng/ml no significant differentiation can be observed. The presence of EGF in the medium is not necessary for assessing the biomarkers EGFR (see example 7).

Example 11: Oligonucleotide Effects on EGFR mRNA in PTEC-TERT1 Cells

Compound 20-1, is also known as ISIS, 388626 is an antisense oligonucleotide comprising 2′-O-methoxyethyl-RNA (MOE) modifications, targeting sodium-glucose co-transporter 2 (SGLT2). This compound has been shown to cause reversible in vivo nephrotoxicity in humans when dosed weekly at 50 mg, 100 mg or 200 mg in a 13 week study (Meer et al 2016 J Pharmacol Exp Ther Vol 359 pp 280-289).

In the present example it was investigated whether this nephrotoxicity could be predicted by measuring EGFR mRNA upon administration of compound 20-1 to PTEC-TERT1 cells.

The primary immortalized PTEC-TERT-1 cell line was cultured according to the conditions described in the “Materials and methods” section. At confluence the cells were treated with oligonucleotide as described in the “Materials and methods” section, in concentrations of 30, 100, 300, 400 or 500 μM.

The EGFR mRNA was measured using the assays described in the “Materials and methods” section.

The results are shown in tables 12 below and represent the average of three identical treatments.

TABLE 12 EGFR mRNA 9 days after oligonucleotide treatment of PTEC-TERT1 cells Day 9 Conc EGFR μM % saline SD saline 100 12  30 90 16 100 72 8 300 61 5 400 59 7 500 60 13

From these data it can be seen that the in vivo nephrotoxicity of the MOE antisense oligonucleotide (compound 20-1) could be predicted using PTEC-TERT1 cells with EGFR mRNA as biomarker at oligonucleotide concentrations above 100 μM. 

The invention claimed is:
 1. A method for selecting one or more nucleic acid molecules with a reduced in vivo nephrotoxicity profile selected from the group consisting of a RNAi agent, an antisense oligonucleotide and an aptamer for in vivo administration to a mammal, from a library of nucleic acid molecules, said method comprising the steps of a. obtaining a library of nucleic acid molecules; b. administering each member of the library of nucleic acid molecules to a cell culture expressing epidermal growth factor receptor (EGFR); c. culturing the cells in vitro in a culture media for a period of time; d. measuring the amount of intracellular EGFR mRNA, and optionally additional biomarkers, for each nucleic acid molecule; and e. selecting one or more nucleic acid molecules wherein the % reduction in EGFR relative to a reference value is above 80%, wherein the selected molecules have a reduced in vivo nephrotoxicity profile.
 2. The method according to claim 1, wherein the therapeutic index of the selected nucleic acid molecule is decreased when compared to a toxic reference substance or parent nucleic acid molecule.
 3. The method according to claim 1, wherein the library of nucleic acid molecules is a library of nucleic acid molecule variants (child nucleic acid molecules) of a parent nucleic acid molecule, wherein the parent nucleic acid molecule is nephrotoxic, and wherein step d) identifies one or more nucleic acid molecule variants which are less nephrotoxic than the parent nucleic acid molecule; wherein the nucleic acid molecule variants retain the nucleobase sequence of the parent nucleic acid molecule.
 4. The method according to claim 1, wherein EGFR mRNA level is compared to a reference value obtained from cells treated with vehicle control or a non-toxic reference nucleic acid molecule, where the non-toxic reference nucleic acid molecule has been validated as non-toxic in vivo.
 5. The method according to claim 4, wherein the non-toxic reference nucleic acid molecule is an antisense oligonucleotide compound consisting of CGTcagtatgcgAATc (SEQ ID NO: 1), wherein lower case letters represent DNA units, bold upper case letters represent beta-D-oxy-LNA units, all LNA C are 5′methyl C and all internucleoside linkages are phosphorothioate linkage.
 6. The method according to claim 5, wherein a level of EGFR mRNA below 80% relative to the vehicle control or non-toxic reference value is predicative of nephrotoxicity of the nucleic acid molecule.
 7. The method according to claim 4, wherein EGFR mRNA level is further compared to a second reference value obtained from cells treated with a nephrotoxic reference nucleic acid molecule, where the nephrotoxic reference nucleic acid molecule has been validated to cause nephrotoxicity in vivo.
 8. The method according to claim 7, wherein the toxic reference nucleic acid molecule is an antisense oligonucleotide compound consisting of GCtgtgtgagcttGG (SEQ ID NO: 4), wherein lower case letters represent DNA units, bold upper case letters represent beta-D-oxy-LNA units, all LNA C are 5′methyl C and all internucleoside linkages are phosphorothioate linkage.
 9. The method according to claim 1, wherein step d) further comprises the measurement of extracellular kidney injury molecule-1 (KIM-1) protein or intracellular mRNA levels, wherein an increase in KIM-1 levels are indicative of a nucleic acid molecule which is, or is predicted to be, associated with nephrotoxicity.
 10. The method according to claim 9, wherein a level of KIM-1 protein above 200% relative to the saline or non-toxic reference value is predicative of nephrotoxicity of the nucleic acid molecule.
 11. The method according to claim 9, wherein a level of KIM-1 mRNA above 1000% relative to the saline or non-toxic reference value is predicative of nephrotoxicity of the nucleic acid molecule.
 12. The method according to claim 9, wherein the increase in KIM-1 is predicative of nephrotoxicity for a nucleic acid molecule even if the EGFR mRNA level is not decreased.
 13. The method according to claim 1, wherein the culture media in step a) comprises at least 4 ng/ml of epidermal growth factor (EGF) and step d) further comprises the measurement of intracellular adenosine triphosphate (ATP) levels; wherein a decrease in intracellular ATP levels is indicative of a drug substance which is, or is predicted to be, associated with nephrotoxicity.
 14. The method according to claim 13, wherein a level of intracellular ATP less than 80% of the saline or non-toxic reference value is predicative of nephrotoxicity of the drug substance.
 15. The method according to claim 1, wherein the cells expressing EGFR is selected from the group consisting of epithelial cell, endothelial cell and mesenchymal cells, and neuroectodermal cells.
 16. The method according to claim 15, wherein the cell culture is a primary kidney epithelial cell culture selected from the group consisting of proximal tubule epithelial cells, distal tubule epithelial cells and collecting duct epithelial cells, primary human PTEC or rat PTEC cells.
 17. The method according to claim 15, wherein the cells expressing EGFR are cultured from an immortalized cell line of human PTEC-TERT-1, ciPTEC, CACO2, HK-2, NKi-2 or human A549 cell lines.
 18. The method according to claim 1, wherein the period of incubation with the nucleic acid molecule is between 2 and 6 days, or around 3 days.
 19. The method according to claim 1, wherein the nucleic acid molecule comprises one or more 2′ sugar modified nucleosides, independently selected from the group consisting of 2′-O-alkyl-RNA, 2′-O-methyl-RNA, 2′-alkoxy-RNA, 2′-O-methoxyethyl-RNA, 2′-amino-DNA, 2′-fluoro-DNA, arabino nucleic acid (ANA), 2′-fluoro-ANA and LNA nucleosides.
 20. The method according to claim 1, wherein the nucleic acid molecule comprises at least one modified internucleoside linkage.
 21. The method according to claim 1, wherein the nucleic acid molecule is an antisense oligonucleotide capable of recruiting RNase H.
 22. The method according to claim 1, wherein the nucleic acid molecules are targeted to a selected gene that is not EGFR.
 23. The method according to claim 1, wherein the nucleic acid molecules are not complementary to EGFR mRNA and have at least 3 mismatches to EGFR mRNA. 